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Article
Solution NMR structure of GATase subunit and structural basis of interaction between GATase and ATPPase subunits in a two-subunit-type GMPS from Methanocaldococcus jannaschii Rustam Ali, Sanjeev Kumar, Hemalatha Balaram, and Siddhartha Peddibhotla Sarma Biochemistry, Just Accepted Manuscript • DOI: 10.1021/bi400472e • Publication Date (Web): 31 May 2013 Downloaded from http://pubs.acs.org on June 7, 2013
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Biochemistry
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Solution NMR structure of GATase subunit and structural basis of interaction between GATase
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and ATPPase subunits in a two-subunit-type GMPS
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from Methanocaldococcus jannaschii
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Rustam Ali1, Sanjeev Kumar2, Hemalatha Balaram2 and Siddhartha P. Sarma1*
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1
Molecular Biophysics Unit, Indian Institute of Science, Bangalore, Karnataka-560012, INDIA.
2
Molecular Biology and Genetics Unit, Jawaharlal Nehru Center for Advanced Scientific Research, Bangalore-560064, Karnataka, INDIA.
Address Correspondence to Siddhartha P Sarma 207 Molecular Biophysics Unit Indian Institute of Science Bangalore – 560012 Karnataka, INDIA E-mail:
[email protected] Tel: 918022932839 Fax: 918023600535
20 21
The authors would like to thank the Department of Science and Technology and the Department
22
of Biotechnology, Government of India for the NMR and Mass spectrometric facilities at the
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Indian Institute of Science. HB acknowledges Department of Biotechnology and Department of
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Science and Technology, Government of India for funding.
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Rustam Ali is grateful to the Indian Institute of Science for a doctoral fellowship. Sanjeev Kumar
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was a recipient of CSIR Junior Research and Senior Research fellowships.
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Keywords:
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de-novo purine nucleotide biosynthesis; solution NMR; fast chemical exchange; intermediate
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chemical exchange; glutamine amidotransferase; guanosine monophosphate synthetase; protein –
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ligand interaction; protein – protein interaction; amination; ammonia channeling.
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1
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ATP, Adenosine Triphosphate; ATPPase, ATP pyrophosphatase; DSS, Sodium 4,4-Dimethyl-4-
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Silapentane Sulfonate; ESI-MS, Electrospray Ionization Mass Spectrometry; GAT, Glutamine
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dependent
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Amidotransferase; GMP, Guanosine monophosphate; GMPS, Guanosine monophosphate
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Synthetase;
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Imidazoleglycerolphosphate synthase; MALDI - TOF, Matrix Assisted Laser Desorption
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Ionization – Time of Flight; Mj GATase, Methanocaldococcus jannaschii GATase; Mj GMPS,
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Methanocaldococcus jannaschii GMPS; NAD, Nicotinamide adenine dinucleotide; NMR,
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Nuclear magnetic resonance; NOE, Nuclear Overhauser Effect; NOESY, Nuclear Overhauser
45
effect spectroscopy; Ph, P. horikoshii; XMP, Xanthosine monophosphate; rmsd, root mean
46
square deviation.
Abbreviations:
amidotransferase;
HSQC,
GDH,
Glutamate
Heteronuclear
Single
dehydrogenase;
Quantum
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GATase,
Coherence;
Glutamine
IGPS,
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Abstract:
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Methanocaldococcus janaschii (Mj) guanosine monophosphate synthetase (GMPS) has been
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determined using high-resolution nuclear magnetic resonance methods. Gel filtration
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chromatography and
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present in solution as a 21 kDa (188 residues) monomer. The ensemble of twenty lowest energy
64
structures showed an rmsd of 0.35±0.06 Å for backbone and 0.8±0.06 Å for all heavy atoms.
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Furthermore, 99.4 % backbone dihedral angles are present in allowed region of the
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Ramachandran map, indicating the stereochemical quality of the structure. The tertiary structure
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of the GATase is composed of a seven-stranded mixed β-sheet that is fenced by five α-helices.
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The Mj GATase is similar in structure to the Pyrococcus horikoshi (Ph) GATase subunit. NMR
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chemical shift perturbation and changes in line width were monitored to identify residues on
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GATase that were responsible for interaction with magnesium and the ATPPase subunit
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respectively. These interaction studies showed that a common surface exists for the metal-ion
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binding as well as for the protein–protein interaction. The dissociation constant for the GATase-
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Mg2+ interaction has been found to be ~1 mM, which implies that interaction is very weak and
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falls in fast chemical exchange regime. The GATase-ATPPase interaction on the other hand
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falls in intermediate chemical exchange regime on NMR time scale. The implication of this
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interaction on the regulation of the GATase activity of holo GMPS is discussed.
The solution structure of the monomeric glutamine amidotransferase (GATase) subunit of the
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N backbone relaxation studies have shown that Mj GATase subunit is
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Protein–protein interactions are at the core of most of the physiological process (1-3).
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Enzymes have been evolved to carry out a chemical reaction in an efficient and concerted
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manner. Guanosine monophosphate synthetase (4), presents the special example of a coupled
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enzyme catalyzed reaction where the component reactions are carried out by two distinct
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domains/subunits.GMPS1 a class I glutamine amidotransferase (5, 6), is an important enzyme
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that catalyzes the final step of GMP biosynthesis. Two reactions are catalyzed by the GMPS
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enzyme; 1) the hydrolysis of glutamine to yield ammonia and 2) amination of XMP to yield
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GMP (7, 8). The overall reaction is ATP dependent and requires Mg2+. The enzyme thus contains
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two independent catalytic sites that could either be housed in individual domains in a single
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polypeptide chain, or in separate subunits, and are known as the GATase and ATPPase domains
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or subunits respectively. In eukaryotes, bacteria and some archaea GMPSs are encoded for by a
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single gene (two-domain-type). In most other archaeal species, e.g., M. jannaschii, the GATase
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and ATPPase functions are present on individual polypeptides (two-subunit-type) that are coded
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for by separate genes. GATase catalyzes the hydrolysis of glutamine and ATPPase uses the
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ammonia generated to convert XMP to yield GMP. GMP formation occurs via a nucleophilic
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attack by the released ammonia on the adenyl-XMP intermediate (9-11).
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A PDB query for GMPS gives eleven hits. All structures have been solved by X-ray
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crystallography. These structures belong to GMPS from P. falciparum, H. sapiens, T.
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thermophilus, C. burnetii, P. horikoshii and E. coli. Except for P. horikoshii all GMPSs are two-
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domain-type. An analysis of different crystal structures from PDB reveals that the core structural
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elements are highly similar in GMPS. The GATase domain/subunit contains α/β structures. The
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core of the structure is formed by mixed β-sheet mainly constructed from parallel β-strands. The
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catalytic triad is conserved across these enzymes. The catalytic triad of GATase appears similar 4 ACS Paragon Plus Environment
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to those in serine proteases, however, with serine being replaced by cysteine and aspartate by
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glutamate in GATase.
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The ATPPase domain/subunit of GMPS has a typical dinucleotide binding site which
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resembles dehydrogenases. This fold is made up of five stranded sheets sandwiched between α-
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helices. ATPPase has a signature nucleotide-binding motif or P-loop that is highly conserved in
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all the nucleotide binding proteins (12). X-ray crystal structures of single-chain GMPSs have
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shown that the glutamine and XMP binding sites are separated by a distance of 10-40 Å. Thus,
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the ammonia released at glutamine binding site has to be channeled to the acceptor or ATPPase
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site (12-14). Ammonia channeling is the hallmark of a large group of proteins known generally
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as glutamine dependent amidotransferases, of which the GMPSs form one sub-group (7, 12, 14,
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15). This ammonia channeling and cross talk between two domains have been a major thrust of
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investigation in glutamine amidotransferases. Most of the studies have been carried out on two-
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domain-type GMPS (12, 16-21), while only one study has been reported from two-subunit-type
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GMPS (22).
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The GMPS from Methanocaldococcous jannaschii is a two-subunit-type GMPS. The
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glutamine amidotransferase (GATase) subunit of M. jannaschii is a monomer of molecular
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weight of 21 kDa, whereas the ATPPase subunit is a dimer with each protomer having a
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molecular weight of 34 kDa. There are several open questions with regard to the functioning of
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this enzyme. Unlike regular enzymes GATs are bi-enzymes and therefore function through the
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formation of protein-protein complexes that is facilitated by ligand binding to the synthase
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domain. Further, their activities are tightly coordinated leading to maximization of overall
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catalytic efficiency. Interestingly, different GATs seem to adopt different molecular mechanisms
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and thus the molecular mechanism that co-ordinate the various events warrants investigation. 5 ACS Paragon Plus Environment
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Recent studies have shown that GATase subunit interacts with ATPPase only when the
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latter is fully liganded and furthermore, the glutaminase activity is tightly regulated by
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interaction between GATase and ATPPase subunits (22). In the case of M. jannaschii GMPS,
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the ATPPase subunit alone is capable of catalyzing the hydrolysis of ATP. On the other hand the
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GATase does not show glutaminase activity in the absence of fully liganded ATPPase subunit.
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Our interest lies in understanding the structural basis for the interaction between the GATase and
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ATPPase subunits and the role of this important interaction in catalyzing the formation of GMP.
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To date, there is no structural information available for the two-subunit-type GMPS holoenzyme.
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Also, poorly understood are the conformational changes in GATase subunit upon interaction
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with liganded ATPPase that lead to its activation. In order to gain a better understanding of the
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mechanistic principles, we initiated structural studies of M. jannaschii GMPS. As a first step we
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have determined the solution structure of the Mj GATase subunit by high-resolution multinuclear
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NMR spectroscopy. We have also studied the interaction of GATase with the co-factor Mg2+ and
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interaction between Mj GATase and ATPPase subunit.
141 142
Materials and Methods
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Over-expression and purification
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The expression and purification of the Mj GATase subunit of M. jannaschii has been
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described earlier (23). Isotopically enriched (13C,
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prepared using
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respectively (24). Gene for ATPPase subunit from M. jannaschii genomic DNA was cloned into
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pET3atr using NdeI and BamH1restriction sites, and subcloned into cassette III of pST39
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expression vector using Sac I and Kpn restriction sites. Plasmids carrying gene for ATPPase
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C6-glucose and
15
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N or
15
N) samples of Mj GATase were
NH4Cl or 15NH4Cl as the sole source of carbon and nitrogen
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subunit were transformed into Rosetta (DE3) pLysS E. coli over-expression strain. Mj ATPPase
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subunit was over-expressed and purified using the same protocol as described for Mj GATase
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subunit.
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Chromatographic studies
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Gel filtration studies were carried out using a Superdex-200 column (10 mm x 300 mm)
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attached to an AKTA Basic HPLC system. The column was equilibrated with 50 mM phosphate
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buffer, pH 7.0. Beta-amylase (200 kDa), alcohol dehydrogenase (150 kDa), bovine serum
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albumin (66 kDa), carbonic anhydrase (29 kDa) and cytochrome c (12.4 kDa) were used for
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molecular weight calibration. The protein samples were eluted at a flow rate of 0.5 ml/min.
160 161
Gel filtration co-chromatography
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The column was pre-equilibrated with buffer (20 mM Tris, pH 7.4)alone or with buffer
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containing appropriate ligands. The concentration of ATP and XMP in the running buffer was
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100 µM each. The concentrations of Mj ATPPase and GATase when used alone or in
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combination were 10 µM each. The concentrations of ATP and XMP used for pre-incubation
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with the enzyme were 3 mM and 0.2 mM, respectively. Equimolar Mj GATase and ATPPase
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were pre-incubated on ice with substrates under four conditions: A) 20 mM MgCl2, B) 20 mM
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MgCl2 + 3 mM ATP, C) 20 mM MgCl2 + 200 µM XMP and D) 20 mM MgCl2 + 3 mM ATP +
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200 µM XMP. These samples were chromatographed. Fractions were collected and analyzed by
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SDS-PAGE.
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Metal affinity co-chromatography
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An N-terminal hexa-histidine tagged Mj GATase was generated in pET21b. This clone was
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verified by DNA sequencing and protein expressed in Rossetta (DE3) pLysS and purified using
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Ni-NTA agarose beads. The protein was passed through a desalting column (Sephacryl-200) and
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concentrated before further use. Mj GATase affinity beads were generated by incubating Ni-
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NTA agarose with 10 µM purified Mj GATase followed by buffer wash to remove unbound
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enzyme. Mj ATPPase (10 µM) was incubated for 15 minutes on ice with 2 mM ATP, 0.2 mM
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XMP in 20 mM Tris buffer, pH 7.4, containing 20 mM MgCl2. The pre-incubated Mj ATPPase
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was mixed with the beads and incubated at 4 ºC for 30 min. The beads were then washed with
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buffer A (20 mM Tris HCl, pH 7.4) and subsequently with buffer B (20 mM Tris HCl, pH 7.4
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containing 3 mM ATP, 0.2 mM XMP, 20 mM MgCl2). The protein was eluted from the column,
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using buffer A solution containing 500 mM imidazole. The column fractions were analyzed by
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SDS-PAGE.
186 187
Biochemical Assay
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Measurement of GATase activity
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Mj GATase activity was monitored by a coupled enzyme assay; wherein glutamate
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formation was coupled to the reduction of NAD+ to NADH by glutamate dehydrogenase and the
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reaction was followed by spectrophotometry. The concentration of NADH was estimated from
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absorbance measurements at 340 nm using a molar extinction co-efficient value of 6220 M-1 cm-1
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(25). The reaction mixture consisted of 100 µM GATase and 100 µM glutamine in 100 mM Tris
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HCl, pH 7.4 and was incubated at either 22 ºC for 30 min or 70 ºC for 15 min. The reaction was
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quenched by boiling for 5 minutes followed by centrifugation at13000 g. The supernatant (100 8 ACS Paragon Plus Environment
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µl) was mixed with 0.5 mM NAD+ and glutamate dehydrogenase (1.8 Units) in a buffer
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containing 50 mM KCl and 1 mM EDTA. The reaction mixture was incubated for 1 hour at 37
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0
199
mutually excluded.
C. Separate control reactions were also carried out wherein GATase and glutamine were
200 201
GATase activity in the presence of ligand bound ATPPase
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The Mj GATase activity was monitored by an assay described in previous section.
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Concentrations of enzymes and ligands used in the assays were 2 µM GATase, 2 µM ATPPase,
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0.2 mM XMP, 2 mM ATP and 5 mM glutamine. Reactions were carried out in a buffer
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containing 100 mM Tris HCl, pH 7.4, 20 mM MgCl2 at 70 ºC for15 min and quenched by
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boiling for 5 minutes.
207 208
Stoichiometry of GATase-ATPPase complex
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Stoichiometry of the GATase-ATPPase complex was determined by monitoring the
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formation of GMP. The reaction mixture contained fixed concentration of 2 µM ATPPase, 3 mM
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ATP, 0.2 mM XMP, 20 mM glutamine and varying concentrations of GATase (0-16 µM). The
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reaction was carried out in 90 mM Tris HCl, pH 7.0, containing 20 mM MgCl2 at 70 ºC. The
213
reactions were initiated with 2 µM Mj ATPPase and varied concentrations of GATase.
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Formation of GMP was monitored spectrophotometrically, by measuring absorbance at 290 nm
215
and the concentration was estimated using a molar extinction co-efficient value of 1500 M-1cm-1
216
(26).
217 218
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NMR spectroscopy
220
Sample preparation
221
Samples for NMR spectroscopy were prepared in 20 mM potassium phosphate buffer pH
222
7.0, containing 2 mM DTT, 0.1 mM EDTA, 1 mM PMSF and 0.01% sodium azide. Three
223
dimensional
224
GATase that were 0.70 mM in 90% H2O/10%D2O or 100% D2O respectively. Nitrogen-15
225
relaxation experiments were recorded using samples of Mj GATase (0.4 mM) in 90% H2O/10%
226
D2O.
15
N-edited and
13
C-edited NMR experiments were recorded using samples of Mj
227 228
Data acquisition
229
NMR data were acquired either on an Agilent 600 MHz spectrometer equipped with a 5
230
mm triple resonance pulsed field gradient (TRPFG) probe or on a Bruker Avance 700 MHz
231
spectrometers equipped with 5 mm TXI triple resonance PFG (z-axis) probe. The sample
232
temperature was maintained at 30 ºC during all experiments. Chemical shifts were referenced to
233
external DSS. Two dimensional 1H-15N HSQC spectra (27) were acquired at 700 MHz using
234
proton spectral widths of 14006 Hz in the acquired dimension and 2129 Hz in the indirectly
235
detected dimension. Water suppression was achieved by using a pulse program that incorporated
236
the WATERGATE (28) solvent suppression scheme. The STATES-TPPI mode of quadrature
237
detection was used for frequency selection in the indirectly detected dimension. The 1H-13C
238
HSQC spectra were acquired at 700 MHz in sensitivity-enhanced mode. Proton and carbon
239
spectral widths of 14006 Hz and 10914 Hz were recorded in the directly detected and indirectly
240
detected dimensions respectively. Frequency discrimination in the indirectly detected dimension
241
was achieved via coherence selection using pulsed field gradients. Water suppression was 10 ACS Paragon Plus Environment
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242
achieved via coherence selection and by the use of using trim pulses. Three-dimensional
243
edited 1H-1H NOESY spectra (mixing time, τm= 150 ms and 200 ms) and
244
NOESY (29) spectra (mixing time, τm = 150 ms) were acquired at 700 MHz using proton
245
spectral widths of 14005.60 Hz and 14005.60 Hz in F3 and F1 dimensions, and nitrogen and
246
carbon spectral width of 2128.65 Hz and 4225 Hz, respectively in the F2 dimension. Data were
247
acquired in phase sensitive mode, using the States-TPPI (15N-edited NOESY) or Echo-AntiEcho
248
method (13C-edited NOESY) of quadrature detection for the indirectly detected dimensions.
13
N-
C-edited 1H-1H
249 250
15
251
T1, T2 measurement
252
Spin–lattice relaxation rate, T1, and spin–spin relaxation, T2, were measured by recording
253
two dimensional 1H-15N HSQC spectra on an Agilent 600 MHz NMR spectrometer equipped
254
with a 5 mm triple resonance pulsed field gradient (TRPFG) probe (30, 31). The sample
255
concentration used for T1 and T2 measurements was 0.4 mM. The data used for T1 measurement
256
were acquired with 2 sec recycle delays and relaxation delays of 10, 50, 100, 250, 400, 550, 750,
257
900 and 1200 ms. T2 data were acquired with 2 sec recycle delays and relaxation delays of 10,
258
30, 50, 70, 90, 110, 130, 150 and 170 ms. T1 and T2 values were determined by fitting peak
259
heights using the nonlinear least-squares routine, using Analysis (32).
N Backbone Dynamics
260
Calculation of Rotational correlation time (τc)
261
Rotational correlation time (τc) was measured using the following formula (30, 33)
262 263
τc = 1/4πνN (6×T1/T2− 7)1/2 where νN is the 15N resonance frequency (in Hz).
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Hydrogen – deuterium exchange
266
A series of 2D 1H-15N HSQC spectra at an interval of 45 minutes over a period of 24 hours,
267
were acquired in 100% D2O. Lyophilized samples of Mj GATase subunit were dissolved in D2O
268
just before data acquisition.
269 270
Data processing and analysis
271
All 2D and 3D NMR data were processed by using NMRPipe/NMRDraw processing
272
software (34) on an Intel PC workstation running Suse Linux 11.3. The directly and indirectly
273
detected time domain data of 2D and 3D spectra were processed by applying a 90° phase-shifted
274
squared sinebell or a Gaussian filter with a line-broadening parameter of 10 Hz as weighting
275
functions. Data sets were zero-filled prior to Fourier transformation. Processed data were
276
analyzed using the ANALYSIS module in CCPN.
277 278
Structure determination
279
Distance and dihedral angle restraints
280
Inter-proton distance restraints were calculated from the intensities of unambiguously
281
assigned NOE correlations in the 3D 15N-edited NOESY-HSQC and
13
282
spectra. On the basis of integrated intensities, NOEs were classified as strong, medium, weak and
283
very weak with upper distance bounds of 2.8, 3.5, 5.0 and 6.0 Å respectively. All distance
284
restraints employed a lower bound of 1.80 Å. Hydrogen bond restraints were generated for
285
residues that were slow to exchange in H/D exchange experiments. The upper distance bound
286
employed for the hydrogen bonds were set to 2.2 Å for HN···O and 3.2 Å for N···O pairs.
287
Backbone dihedral angles phi (φ) and psi (ψ) were predicted using the program TALOS (35)
C-edited NOESY-HSQC
+
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α
13
α
288
using the observed HN, 1H ,
289
allowed during structure calculation.
C ,
13
β
C chemical shifts. An angular variation of ± 30º was
290 291
Solution structure evaluation
292
Three-dimensional structures were calculated using torsion angle dynamics protocol in the
293
program CYANA-3.0 (36, 37). Experimentally derived distances from NOEs, hydrogen-bond
294
distances and dihedral angle restraints were used as input for the structure calculation. A hundred
295
random conformers were subjected to 20000 steps of annealing. An ensemble of twenty lowest
296
energy conformers out of hundred calculated conformers were selected on the basis of target
297
function and which had no upper distance violations greater than 0.2 Ǻ and no dihedral angle
298
violations greater than 5°. The conformer with minimum energy/target function was chosen as a
299
representative conformer. The structures were analyzed using MOLMOL (38). The quality of
300
structure was further assessed by Protein structure validation suit (PSVS) (39). Structure
301
alignment was performed using either DALI (40) or PyMOL (41).
302 303
Interaction studies
304
Interaction with the cofactorMg2+
305
Perturbations in chemical shift of residues in Mj GATase, as observed in 1H-15N HSQC
306
spectra, upon interaction with Mg2+, were followed by NMR titration studies.
307
GATase (50 µM) was titrated with varying concentration of MgCl2 (0.5 mM–20 mM). Chemical
308
shift perturbation as a function of MgCl2 concentration in HSQC spectrum was used to calculate
309
dissociation constant (Kd). Weighted chemical shift change per residue (∆) was calculated by the
310
equation (42); 13 ACS Paragon Plus Environment
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N-enriched Mj
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∆ = [(δH)2 + (0.1δN)2]1/2
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(2)
312
where δH and δN are changes in chemical shifts of 1HN and
313
constant for the interaction was determined by plotting the ∆ as a function of increasing MgCl2
314
concentration. The resulting curve was fitted into the following equation
315
15
N, respectively. Dissociation
∆ = ∆max([L]T + [P]T + Kd - {([L]T + ([P])T + Kd)2 - 4[L]T[P]T}1/2)
(3)
316
where ∆ is the observed chemical shift change at a given total ligand concentration, [L]T,
317
(relative to the resonance frequency in absence of MgCl2), ∆max is the change in chemical shift at
318
saturation and [P]T is the total protein concentration (43-47).
319 320
Interaction with ATPPase
321
A method, similar to the one described in the previous section was used to study the
322
interaction between Mj GATase and Mj ATPPase subunits. Nitrogen-15 labeled Mj GATase (50
323
µM) was titrated with varying concentration of unlabeled Mj ATPPase (20 µM to 160 µM), in
324
presence of saturating concentration of all substrates viz; MgCl2 (20 mM), ATP (8 mM) and
325
XMP (2 mM). All the experiments were carried out in a 40 mM potassium-phosphate buffer, pH
326
7.0, containing 50 mM NaCl. The control experiment was recorded on 15N enriched Mj GATase
327
(50 µM) sample in presence 20 mM MgCl2, 8 mM ATP and 2 mM XMP. To this, varying
328
concentration of unlabeled Mj ATPPase (20 µM to 160 µM) was added. Each titration
329
experiment was started on a freshly prepared sample to avoid a dilution effect upon addition of
330
ligand. All samples were prepared from the same stock solutions. Data were recorded by placing
331
the sample in a 5 mm, deuterium susceptibility matched Shigemi tube (Pennsylvania, USA). The
332
total sample volume used in a Shigemi tube was kept constant at 300 µl. The concentration of
333
stock solutions of Mj GATase and Mj ATPPase were 0.43 mM and 0.53 mM respectively. The 14 ACS Paragon Plus Environment
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Biochemistry
334
Mj GATase and Mj ATPPase protein concentrations were measured on a NanoDrop 1000
335
spectrophotometer using molar extinction coefficient values of 15930 M-1cm-1 and 22190 M-
336
1
337
intensity (I0). The decrease in intensity due to line broadening/chemical exchange contribution to
338
the relaxation, arising from interaction between two subunits was determined by measuring peak
339
height. Change in intensity (∆I) upon ligand binding was calculated as
cm-1 respectively. The intensity of a resonance in the control experiment was taken as reference
∆I = I0 – I
340
(4)
341
where I0 is the peak intensity in absence of ligands in control experiment and I represents peak
342
intensity in presence of ligand, analogous to the approach used by (48). The data was normalized
343
with respect to reference intensity (I0). The intensity of a resonance that disappeared on titration
344
with ATPPase subunit was taken as zero. The calculated ∆Inormalized was plotted against residue
345
number. A cut off of 0.8 was set for the residue interacting directly with Mj ATPPase subunit
346
while a cut off ≥ 0.75 but less than 0.8 was set for the residues those interacting indirectly. The
347
residues involved in interaction with Mj ATPPase subunit were mapped onto the calculated
348
solution NMR structure of Mj GATase.
349 350
H/D exchange studies
351
In an effort to identify interface residues in the Mj GATase-ATPPase complex, H/D
352
exchange NMR experiments were also carried out. Sample for control experiment was prepared
353
by lyophillization of 50 µM Mj GATase. Equivalent amounts of powdered MgCl2, ATP and
354
XMP were added and the mixture was dissolved in D2O, just prior to data acquisition. The final
355
concentrations of MgCl2, ATP and XMP in the solution were 20 mM, 8 mM and 2 mM
356
respectively. Similarly, Mj GATase (50 µM) and ATPPase (50 µM) were co-lyophillized and 15 ACS Paragon Plus Environment
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357
subsequently equivalent amount of powdered form of MgCl2, ATP and XMP were added. D2O
358
was added just before data acquisition. 1H-15N HSQC spectra were acquired as described above.
Page 16 of 66
359 360
Reaction assay
361
All reaction assays were carried out in 20 mM phosphate (pH 7.0) buffer at 303 K. The
362
reaction mixture contained 5 µM Mj GATase, 5 µM Mj ATPPase, 20 mM MgCl2, 2 mM ATP,
363
240 µM XMP and 20 mM Glutamine. The substrates and co-factors were mixed. The reaction
364
was initiated by the addition of enzymes and this reaction mixture was transferred into a NMR
365
tube. Time course of the reaction was followed by recording one-dimensional proton NMR
366
spectra. GMP formation was tracked by monitoring the H8, 6NH2 and H1' resonances of GMP,
367
which are known to occur at 8.3 ppm, 6.3 ppm and 5.8 ppm respectively. Chemical shifts were
368
referenced to internal DSS. In a similar manner, formation of AMP was monitored by tracking
369
H8 resonance of AMP at 8.55 ppm. GATase and glutamine were excluded from the reaction
370
mixture, where only AMP formation was monitored. Spectra were recorded at intervals of 10
371
minutes, processed and analysed.
372 373
Results
374
Solution properties of Mj GATase
375
Figure 1 shows the gel filtration chromatography elution profile when the Mj GATase
376
subunit is passed through a Superdex-200 gel filtration column. Comparison of the elution
377
volume (Ve) of Mj GATase with those of proteins of known molecular weight showed that Mj
378
GATase behaves as a monomer in solution with a molecular weight of ~ 21 kDa. In light of this,
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Biochemistry
379
the protocols followed for structure determination were those that were generally applicable for
380
monomeric proteins.
381 382
NMR spectroscopy
383
Sequence specific assignment and secondary structure
384
Figure 2 shows the sequence specifically assigned 1H-15N HSQC of the GATase subunit of
385
Mj GMPS. The sequential connectivity assignments obtained from analysis of the three-
386
dimensional 15N-edited NOESY-HSQC spectrum for residues 35 to 40 are shown in figure 3. A
387
summary of the sequential and short range NOEs between backbone atoms and side chain and
388
backbone atoms is shown in Figure S1 (Supplementary Information). The Mj GATase subunit
389
consists of eleven β-strands and five α-helices. Assignment of sequential, short and medium
390
range NOEs provided corroborative evidence for the secondary structure determined from 1H
391
and
392
sequence number and its comparison with the secondary structure of GATase subunit from P.
393
horikoshii, has been listed in table S1 (Supplementary information) (23).
13
α
C ,
13
β
C secondary chemical shifts. Distribution of secondary structure as a function of
394 395
Three dimensional Structure
396
The three dimensional structure of Mj GATase was determined using NMR derived
397
distance, dihedral and hydrogen bond restraints. The number and type of restraints used for
398
structure calculation are listed in table 1. The table also shows the structural parameters derived
399
for the twenty lowest energy structures. Figure 4a shows the superposition of twenty lowest
400
energy conformers of Mj GATase subunit when superimposed on their backbone (N, C, and C )
α
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Page 18 of 66
α
401
atoms. The rmsd, when superposed on the backbone (N,C and C ) atoms and on all heavy atoms,
402
with respect to their mean coordinate position, were 0.35±0.06 Å and 0.8±0.06 Å respectively.
403
An analysis of the backbone dihedral angles in the ensemble of calculated structures shows that
404
99.4 % backbone dihedral angles are present in allowed region of the Ramachandran map (49,
405
50). The low rmsd values for backbone and heavy atoms of all residues (1-188), and the high
406
percentage of residues occupying the allowed regions in the Ramachandran map, indicate that
407
the quality of calculated structure is good. Figure 4b shows the lowest energy conformer of Mj
408
GATase in ribbon representation. The core of the GATase structure is a mixedβ-sheet formed by
409
sevenβ-strands. This mixed β-sheet is made up almost entirely of parallel β-strands, except the
410
β-strand XI, which is anti-parallel in orientation to both strands IX and X. This arrangement
411
makes the mixed β-sheet appear as though it is made up of one β-sheet consisting of five parallel
412
strands and one β-sheet made up of two anti-parallel strands. The first and last β-strands of the
413
core β-sheet are twisted. The core β-sheet is flanked on both sides by five α-helices. The
414
catalytic Cys76, is the only residue with backbone dihedral angles that is present in the
415
disallowed region of the Ramachandaran map. This residue is present at the end of a β-strand
416
and beginning of an α-helix. A similar structural feature has been also observed in other α/β
417
hydrolases (51) (peroxidases, esterases etc.), where the nucleophilic residue is present in a tight
418
α/β turn called “nucleophilic elbow”. Presence of this nucleophilic elbow forces the catalytic
419
residue to populate the disallowed region in the Ramachandaran map.
420 421 422
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Biochemistry
423
Comparison withGATase of Pyrococcus horikoshii
424
The GATase subunit of Mj GMPS and that of Ph GMPS share a 56 % sequence identity.
425
The distribution of secondary structural elements as a function of sequence in Mj GATase is
426
similar to that observed in the X-ray structure of the GATase subunit of the Ph GMP synthetase
427
(52) (PDB ID 2D7J). Figure 5 shows a backbone superposition of these two structures.
428
Significant differences are found only for residues in β-strands V, VI, VII and VIII, which are
429
shorter in length in the solution structures. Additionally, residues 68–70, which are present in a
430
310-helix in the crystal structure, exist in a coil-like conformation in the solution structure. These
431
differences could be attributed to the local dynamics. The Mj and PhGATase are structurally
432
similar to the GATase in two-domain-type GMPS.
433 434
15
435
Figure 6 shows the measured15N T1 and T2 relaxation times for Mj GATase, as a function
N backbone dynamics
15
436
of residue number. The average values of
N T1 and T2 for GATase polypeptide backbone
437
nitrogen atoms are 0.650 ± 0.03 and 0.089 ± 0.003s, respectively. The residues in α-helices and
438
β-sheets exhibit a tight distribution of T1 and T2 values. This is an indication of well- structured
439
regions and corroborates well with the calculated solution structure. On the other hand residues
440
in loop regions show wider distribution of T1. The residues present in loops showed a lower than
441
average value of T2, e.g., G51and G52.
442
Using the average values of T1 and T2, the average global rotational correlational time τc,
443
was found to be ~8.0 ns. The observed value is lower than what one could expect for a 21 kDa
444
molecule (i.e., 10.5 ns).
445 19 ACS Paragon Plus Environment
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446
Page 20 of 66
Biochemical studies
447
Substrate liganded ATPPase is required for Mj GATase activity
448
Mj GATase, in absence of ligand bound ATPPase subunit is inactive. In the presence of
449
substrate liganded ATPPase, viz., Mg2+, ATP and XMP, Mj GATase shows glutaminase activity.
450
A quantitative estimate of this glutaminase activity is shown in Figure 7a. Figure 7b shows the
451
one-dimensional NMR spectra of the conversion of XMP to GMP as a function of time. The
452
resonance lines at δ 5.9 ppm and 5.92 ppm and those at 8.12 ppm and 8.18 ppm correspond to
453
the H1' and H8 protons of XMP and GMP respectively. The resonance line at 6.35 ppm
454
corresponds to that of amino protons of GMP. The decrease in intensity of resonance lines of
455
XMP with the concomitant increase in intensity for resonance lines of GMP is unequivocal proof
456
for the conversion of XMP to GMP. Similar changes in intensity, of resonance lines of ATP and
457
AMP can also be observed. The decrease in intensity of the resonance lines of glutamine is not
458
apparent due to the large stoichiometric excess of this substrate in the reaction mixture. A similar
459
NMR study of GATase alone shows no discernable decrease in the amount of glutamine as a
460
function of time (data not shown). Mj ATPPase, on the other hand is catalytically active even in
461
the absence of GATase subunit. Figure 8 shows that the concentration of XMP (δ 5.90, 8.12)
462
remains unchanged, while that of AMP (δ 8.55 ppm) increases as a function of time.
463 464
Stoichiometry of GATase and ATPPase in the GMPS complex
465
Figure 9 shows the result of Mj ATPPase titration with varying concentration of Mj
466
GATase. A maximum GMP synthetase activity was observed at GATase-ATPPase ratio 1,
467
indicating the stoichiometry of functional of Mj ATPPase-GATase in a functional Mj GMPS is
468
1:1. 20 ACS Paragon Plus Environment
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469
Biochemistry
Interaction studies
470
Interaction between GATase and cofactor Mg2+
471
Binding of Mg2+ to the Mj GATase subunit was studied by NMR spectroscopy. A
472
concentration dependent perturbation of chemical shifts was observed for several residues in the
473
protein. An overlay of the HSQC spectra of Mg2+ free GATase and of Mg2+ saturated15N-
474
labeledMj GATase is shown in figure S2 (Supplementary Information). Figure 10ashows the
475
chemical shift changes in the HSQC spectra for some of the selected residues that are affected by
476
Mg2+ binding. According to Cavanagh et. al., “The near continuous change in chemical shift as a
477
function of increasing Mg2+ concentration is a clear indication that the protein and metal are in
478
a fast chemical exchange regime on NMR time scale”(42). There were no detectable changes in
479
the spectrum at concentrations less than 400 µM and no further change in chemical shift at Mg2+
480
concentrations >10 mM, indicating that protein has reached saturation.
481
The absolute value of the deviation in chemical shift, when compared to the free protein
482
is shown in figure S3 (Supplementary Information). Residues that showed a weighted chemical
483
shift change (∆) greater than 0.05 ppm were considered for calculation of dissociation constant.
484
Twelve residues were showing ∆ greater than 0.05 ppm. Upon mapping these residues on the
485
solution structure of Mj GATase subunit, all residues showing major chemical shift perturbation
486
were present on one side/face of the structure, around the catalytic residue (Figure10b). Residues
487
close to active site, such as H16, G78, H79, S124, H125, D127 and V166 experience significant
488
chemical shift perturbation. Other residues viz; I5, G9, I28, G88 and A93 also experience
489
measurable perturbation. This could be attributed to changes in conformation induced upon Mg2+
490
binding.
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Page 22 of 66
491
The binding curves for the Mg2+-Mj GATase interaction for some of the selected residues
492
are shown in figure 10c. The dissociation constant, Kd, was calculated using equation 2, and was
493
found to be ~ 1 mM. That the Kd is in the millimolar range indicates that the interaction between
494
GATase and Mg2+ is very weak, and falls in very fast exchange regime on NMR time scale. The
495
implications of Mg2+ binding to GATase are discussed below.
496 497
Interaction between Mj GATase and ATPPase
498
Gel filtration chromatography
499
The gel filtration studies (vide supra) have shown that Mj GATase exists in solution as a 15
500
monomer, with a molecular weight of ~ 21 kDa. Evidence for this also comes from the
N-
501
relaxation studies described above. The gel filtration studies also showed that the Mj ATPPase
502
subunit exists as a dimer of molecular weight of ~ 80 kDa. Figure 11a shows the chromatogram
503
of elution profile of Mj GATase and ATPPase in different conditions. Under the
504
chromatographic conditions used the complex should elute as a distinct peak ahead of ATPPase.
505
However, as this was absent, fractions of the peak corresponding to ATPPase were examined on
506
SDS-PAGE and a low level of GATase was seen in the ATPPase fractions (Figure 11b–11e). To
507
improve the ratio of ATPPase and GATase co-eluting, a pull down experiment was carried out.
508
This yielded greater recovery of the protein-protein complex (Figure 12).
509 510
NMR spectroscopic studies
511
The one dimensional proton NMR spectrum of the interaction of the Mj GATase and
512
ATPPase subunits is shown in figure 13a. An overall broadening of the resonances in Mj
513
GATase can be observed in the spectrum. Broadening of the resonance could arise due to 22 ACS Paragon Plus Environment
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Biochemistry
514
chemical exchange of the components of the complex or due to increase in the rotational
515
correlation time (τc) as a function of the molecular size of the complex. The former would
516
suggest that the complex is in intermediate exchange, while the later would indicate that the
517
complex is in slow exchange. In order to get further insight into the interaction between Mj
518
GATase and ATPPase subunits at atomic level, 1H-15N HSQC spectra of 15N-labeled Mj GATase
519
in presence of varying concentration of unlabeled Mj ATPPase and constant saturating
520
concentration of ATP, Mg+2 and XMP were acquired. Figure 13b shows the ovelay of two 1H-
521
15
522
bind to the Mj ATPPase subunit. However, upon addition of MgCl2, ATP and XMP, a significant
523
reduction in the intensity of the correlation peaks was observed for specific residues in Mj
524
GATase (Figure 13c). The change in intensities for some of the interacting residues with respect
525
to the intensities in control experiment has been shown in figures13d and S4 (Supplementary
526
Information). The molecular weight of the Mj GATase-ATPPAse complex is large (~112 kDa)
527
and therefore, the observed overall reduction in intensity could be attributed to the increased
528
molecular weight. The greater than average reduction in intensity observed for specific residues
529
in Mj GATase,as a function of increasing concentration of Mj ATPPase subunit in presence of
530
all substrates indicate that Mj GATase and ATPPase are in chemical exchange, between bound
531
and unbound forms, at a rate that is intermediate on the NMR time scale.
N HSQC spectra. In the absence of substrates and co-factors the Mj GATase subunit does not
532
A plot of normalized change in intensity, ∆Inormalized, as a function of residue number of Mj
533
GATase subunit is shown in figure 14a. In all, 37 residues showed significant decrease in
534
intensity (∆Inormalized > 0.80) upon Mj ATPPase binding. These residues were identified as those
535
that were directly involved in the interaction between Mj GATase and ATPPase subunits. In
536
addition to these, another set of 27 residues also showed significant decrease in intensity 23 ACS Paragon Plus Environment
Biochemistry
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Page 24 of 66
537
(∆Inormalized ≥ 0.75 ≤ 0.80). The decrease in intensities of these residues is most likely due to
538
secondary effects. The residues of Mj GATase subunit that are involved in interaction and form
539
the interaction surface are listed in Table 2. When mapped ontothe structure of Mj GATase
540
structure, these residues were found to be concentrated in five regions of the structure (Figure
541
14b). The residues stretching from V12 to I22, formα-1 helix, while the other four stretches of
542
the residues are present in loopV, loopVII, loopXI, and loop XIV around catalytic triad (C76,
543
H163 and E165). Figure 14c shows the surface representation of Mj GATase subunit showing
544
residues involved in interaction. Residues involved in direct interaction with Mj ATPPase
545
subunit are shown in blue, while the residues involved in indirect interaction are shown in cyan
546
colored. Interestingly, the catalytic residues C76 and H163 were also showing change in
547
intensity greater than 0.80. We could not evaluate change in intensity of E165 because this cross
548
peak overlaps with V29. This clearly indicates that catalytic residues of Mj GATase also undergo
549
conformational change upon interaction with Mj ATPPase subunit. This probably explains why
550
Mj GATase subunit is inactive in the absence of the ATPPase subunit. Therefore we surmise that
551
this interaction brings about a conformational change, which is transmitted around the catalytic
552
site, leading to the activation of Mj GATase subunit.
553 554
Complex between GATase and ATPPase results from a weak interaction:
555
The stability of the Mj GATase-ATPPase complex was probed by H/D exchange NMR
556
experiments. Figure S5 shows an overlay of HSQC spectra of solutions containing Mj
557
GATaseand ATPPase in the absence (in red) and presence (in blue) of all substrates (induces
558
complexation), both of which were acquired in D2O. The residues in αI are slow to exchange in
559
the both cases, which is not surprising as the backbone amide protons are hydrogen bonded. 24 ACS Paragon Plus Environment
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Biochemistry
560
However, residues in loops exchange rapidly with D2O. Thus the residues in the loop regions are
561
not protected in the complex and it is safe to conclude that the interaction between Mj GATase
562
and ATPPase subunits is a transient one and does not result in a stable complex.
563 564
Discussion
565
The biosynthesis of GMP in most of the archaea is catalyzed by a two-subunit-type
566
GMPS enzyme. On the other hand, higher organisms including eubacteria possess a multi-
567
domain GMPS, which probably arose through gene fusion. While much is known of the structure
568
and kinetic and enzymatic properties of the two-domain-type GMPS, the two-subunit-type is less
569
well characterized. Here we have determined the three-dimensional solution NMR structure of
570
the GATase subunit of a two-subunit-type GMPS from M. jannaschii. The structure shows that
571
the molecule is compact and exhibits an α + β fold. The calculated average global correlation
572
time for the Mj GATase subunit was almost 2.5 ns smaller than the expected average global
573
correlation time. This strongly indicates that the molecule is rigid, tightly packed and tumbles
574
isotropically in solution. H / D exchange studies showed that almost 40 percent of the residues
575
Mj GATase residues are either involved in hydrogen bonding in secondary structure or are
576
buried inside the protein core.
577
During the course of our studies, we had observed that optimal activity of GMPS was
578
achieved only under conditions in which the Mg2+ was present at a concentration that was
579
significantly higher than that essential for charge stabilization of ATP. Similar observations
580
have also been made in the case of the two-domain-type GMPS from P. falciparum (16) and
581
human GMPS (19). Our titration data, for the first time, showed that magnesium interacts with
582
Mj GATase subunit in a site-specific manner. The residues that are perturbed in chemical shift 25 ACS Paragon Plus Environment
Biochemistry
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583
due to interaction with Mg2+, lie on one face of the molecule (figure 10c) and form a ring around
584
the catalytic site. Figure 15 shows the electrostatic surface potential for Mj GATase. The
585
interaction between Mg2+ and Mj GATase is not a case of a non-specific electrostatically driven
586
interaction. This is supported by the fact that several other negatively charged regions, which are
587
present on the surface of Mj GATase are unperturbed in the presence of Mg2+. For instance, the
588
surface of helix II is highly negatively charged (4 out of 6 residues are negatively charged).
589
However, no change in chemical shift for the residues in helix II was observed upon titration
590
with Mg2+, indicating that the metal–protein interaction is a highly specific one. The high value
591
of the dissociation constant indicates that this is a weak interaction. In the case of human and Pf
592
GMPS, the site of Mg2+ binding is as yet unknown.
Page 26 of 66
593
The mechanism by which ammonia is channeled from the GATase to the ATPPase is
594
complex and is poorly understood. Structural studies of two-domain-type GMPS do not show a
595
clear conduit for the passage of ammonia from one domain to the other. The structural basis for
596
subunit association in two-subunit-type GMPS’s is not known. Using high-resolution NMR
597
spectroscopic methods, we have also identified the residues on Mj GATase that are responsible
598
for interaction with the ATPPase subunit. There are eight residues on Mj GATase that are
599
common to the interaction with Mg2+ and ATPPase. These residues showed chemical shift
600
perturbation upon Mg2+ binding as well as reduction in intensity upon interaction with ATPPase
601
subunit. Though the exact role of Mg2+ is not known, the fact that a significant number of
602
residues are involved in Mg2+ binding and that these residues are also involved in interaction
603
with ATPPase, indicates that Mg2+ binding must play an important role. Since Mg2+ can bind to
604
GATase subunit independently, one may postulate that Mg2+ binding may play an important role
605
in charge stabilization of the GATase-ATPPase complex. 26 ACS Paragon Plus Environment
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Biochemistry
606
It is important to note that the Mj GATase-ATPPase interaction takes place only
607
in the presence of substrates. The Mj GATase-ATPPase complex undergoes exchange that is
608
intermediate on the NMR time scale. Evidence for this comes from the fact that correlation peaks
609
of 15N-labeled Mj GATase subunit showed neither chemical shift perturbation nor appearance of
610
new correlation peaks with increasing concentration of ATPPase subunit. This rules out the
611
possibility of a fast chemical exchange regime or a slow exchange chemical regime, respectively.
612
Instead, a significant line broadening effect was observed as function of increasing concentration
613
of ATPPase. This could be attributed to the intermediate chemical exchange between two
614
subunits in Mj GATase-ATPPase complex, on NMR time scale. The intermediate chemical
615
exchange regime is characterized by complete broadening of resonances at approximately half of
616
the saturating concentration of ligand and then reappears, probably at slightly different chemical
617
shifts, at much higher concentration of ligand (42). Given the fact that the apparent molecular
618
weight of Mj GATase increases from 21 kDa to 112 kDa, upon complexation with the ATPPase
619
subunit, it is expected that there will be some contribution to the observed line width from the
620
increased rotational correlation time.
621
Most of the studies on GMPS have shown that glutaminase activity is regulated
622
by interaction between GATase and ATPPase subunits. However a recent study on IGPS (53, 54)
623
from Thermotoga maritima, a two subunit-type-amidotransferase has shown that indeed GAT is
624
independently active and absence of constitutive activity is due to the presence of a plug in the
625
channel in the GAT domain. Removal of plug results in constitutive activity. We therefore
626
checked in Mj GATase for such an independent activity using high equimolar quantities of
627
enzyme and glutamine. No measurable activity was observed when GATase and glutamine were
628
incubated at either 22ºC or 70 ºC. It should be noted that under our assay condition, glutamate 27 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
629
concentrations as low as 5 µM can be reliably measured. Thus it is safe to conclude that Mj
630
GATase has no activity and that its activity seems to be tightly regulated. Our NMR studies have
631
shown that catalytic residues C76 and H163 also undergo conformational change upon Mj
632
GATase-ATPPase interaction. The role of catalytic cysteine in GATase domain has been known
633
to be very important (20, 21, 55, 56). This is strong indication that there are conformational
634
changes at catalytic site upon interaction with ATPPase and that these changes could lead to
635
activation of the Mj GATase subunit.
Page 28 of 66
636
Hydrogen-deuterium exchange data provides valuable information about the
637
physical environment of exchangeable protons, i.e., whether they are present in regions of the
638
molecule that are solvent inaccessible and / or are strongly hydrogen bonded. Residues that are
639
solvent exposed often become protected from solvent when they are part of an intermolecular
640
interface. The rate at which these protons undergo solvent exchange is a measure of the strength
641
of association, particularly when the interaction is between large molecules. The rates of
642
exchange of solvent exposed residues in Mj GATase in the presence and absence of ATPPase
643
were nearly identical. This once suggests that the complex is not in slow exchange, but rather
644
exchanges on a time scale that is intermediate to fast.
645
The residues involved in the interaction with ATPPase are those that are present
646
in helix I and in loops V, VII, XI and XIV. Except for helix I, the residues in the loops are
647
present around the catalytic site. The residues in helix I are V12, H13, R14, V15, H16, R17, S18,
648
L19, K20, Y21, and I22. A survey of protein–protein interaction surfaces has shown that Trp,
649
Arg and Tyr predominate and these are considered as “hot spots”. In addition, His, Ile, Lys, Leu,
650
and Met are also found in high proportion. Helix I is well represented by these “hot spot”
651
residues. It has been shown that protein-protein interaction surfaces are generally uneven and 28 ACS Paragon Plus Environment
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Biochemistry
652
consist of rigid and non-rigid structural elements. Furthermore, ~ 65 % of the core interface is
653
formed by rigid residues (57-59). In our case, a tight distribution of T1 and T2 values for residues,
654
V12 to I22, indicates that this helix is rigid. Additionally, the preponderance of positively
655
charged residues in helix I suggests that electrostatic interactions may play a very important role
656
steering complex formation, which could be stabilized by salt bridges (60).
657
In conclusion, we have determined the solution NMR structure of Mj GATase
658
subunit and have shown its interaction with MgCl2. Most importantly, we have identified the
659
specific residues on Mj GATase that are responsible for interaction with the ATPPase subunit.
660
The interaction between these subunits in a two-subunit-type GMPS has not been established
661
earlier.
662
The interaction between Mj GATase and Mg2+ falls in the fast chemical exchange regime
663
on the NMR time scale. The interaction between Mj GATase and ATPPase subunits fall in
664
intermediate chemical exchange regime on NMR time scale. This implies that ammonia
665
channeling occurs at a rate that is fast compared to the exchange rate of the protein-protein
666
complex.
667 668
Accession numbers
669
The structural coordinates for the twenty low energy structures of Mj GATase have been
670
deposited in the Protein Data Bank, PDB ID 2LXN. The chemical shift assignments for Mj
671
GATase have been deposited in the Biological Magnetic Resonance Bank, BMRB ID 17935.
672
673
29 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
674
Supporting Information available
675
Figures providing corroborative evidence for the data shown in the manuscript are included as
676
Supporting information. This material is available free of cost via the internet at
677
http://pubs.acs.org.
678
30 ACS Paragon Plus Environment
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Biochemistry
679
References:
680
1.
Protein Chem.61, 1-8.
681 682
2.
3.
4.
5.
Massiere, F., and Badet-Denisot, M. A. (1998) The mechanism of glutamine-dependent amidotransferases., Cell Mol Life Sci.54, 205-222.
689 690
Zalkin, H., and Murphy, T. (1975) Utilization of ammonia for tryptophan synthesis, Biochem Biophys Res Commun.67, 1370-1377.
687 688
Reichman, D., Rahat, O., Cohen, M., Neuvirth, H., and Schreiber, G. (2007) Molecular architecture of protein-protein binding sites., Curr Opin Struct Biol.17, 67-76.
685 686
Jones, S., and Thornton, J. M. (1996) Principles of protein-protein interactions., Proc Natl Acad Sci USA.93, 13-20.
683 684
Janin, J., and Wodak, S. J. (2002) Protein molecules and protein-protein interactions, Adv
6.
Schendel, F. J., Mueller, E., Stubbe, J., Shiau, A., and Smith, J. M. (1989)
691
Formylglycinamide ribonucleotide synthetase from Escherichia coli: cloning,
692
sequencing, overproduction, isolation, and characterization., Biochemistry28.
693
7.
309.
694 695
8.
Zalkin, H., and Smith, J. L. (1998) Enzymes using glutamine as an amide donor, Adv Enzymol Relat Areas Mol Biol.72, 87-144.
696 697
Zalkin, H. (1993) The amidotransferases, Adv Enzymol Relat Areas Mol Biol.66, 203-
9.
Fukuyama, T. T. (1966) Formation of an adenyl xanthosine monophosphate intermediate
698
by xanthosine 5'-phosphate aminase and its inhibition by psicofuranine, J Biol Chem.241,
699
4745-4749.
31 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
700
10.
von der Saal, W., Anderson, P. M., and Villafranca, J. J. (1985) Mechanistic
701
investigations of Escherichia coli cytidine-5'-triphosphate synthetase. Detection of an
702
intermediate by positional isotope exchange experiments., J. Biol Chem.260, 5343-5350.
703
11.
von der Saal, W., Crysler, C. S., and Villafranca, J. J. (1985) Positional isotope exchange
704
and kinetic experiments with Escherichia coli guanosine-5'-monophosphate synthetase,
705
Biochemistry24, 5343-5350.
706
12.
Tesmer, J. J., Klem, T. J., Deras, M. L., Davisson, V. J., and Smith, J. L. (1996) The
707
crystal structure of GMP synthetase reveals a novel catalytic triad and is a structural
708
paradigm for two enzyme families, Nat Struct Biol.3, 74-86.
709
13.
ammonia-channeling glutamine amidotransferases, Curr Opin Struct Biol.17, 653-664.
710 711
14.
15.
16.
Bhat, J. Y., Shastri, B. G., and Balaram, H. (2008) Kinetic and biochemical characterization of Plasmodium falciparum GMP synthetase, Biochem J.409, 263-273.
716 717
Huang, X., Holden, H. M., and Raushel, F. M. (2001) Channeling of substrates and intermediates in enzyme-catalyzed reactions, Annu Rev Biochem.70, 149-180.
714 715
Raushel, F. M., Thoden, J. B., and Holden, H. M. (2003) Enzymes with molecular tunnels, Acc Chem Res.36, 539-548.
712 713
Mouilleron, S., and Golinelli-Pimpaneau, B. (2007) Conformational changes in
17.
Bhat, J. Y., Venkatachala, R., and Balaram, H. (2011) SUbstrate-induced conformational
718
changes in Plasmodium falciparum guanosine monophosphate synthetase, FEBS J.278,
719
3756-3768.
720
18.
Bhat, J. Y., Venkatachala, R., Singh, K., Gupta, K., Sarma, S. P., and Balaram, H. (2011)
721
Ammonia Channeling in Plasmodium falciparum GMP Synthetase: Investigation by
722
NMR Spectroscopy and Biochemical Assays., Biochemistry50, 3346-3356. 32 ACS Paragon Plus Environment
Page 32 of 66
Page 33 of 66
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
723
Biochemistry
19.
synthetase, J Biol Chem.270, 7347-7353.
724 725
Nakamura, J., and Lou, L. (1995) Biochemical characterization of human GMP
20.
Nakamura, J., Straub, K., Wu, J., and Lou, L. (1995) The glutamine hydrolysis function
726
of human GMP synthetase. Identification of an essential active site cysteine, J Biol
727
Chem.270, 23450-23455.
728
21.
coli guanosine 5'-monophosphate synthetase., J Biol Chem.252, 5431-5436.
729 730
Zalkin, H., and Truitt, C. D. (1977) Characterization of the glutamine site of Escherichia
22.
Maruoka, S., Horita, S., Lee, W. C., Nagata, K., and Tanokura, M. (2010) Crystal
731
structure of the ATPPase subunit and its substrate-dependent association with the
732
GATase subunit: a novel regulatory mechanism for a two-subunit-type GMP synthetase
733
from Pyrococcus horikoshii OT3, J Mol Biol.395, 417-429.
734
23.
Ali, R., Kumar, S., Balaram, H., and Sarma, S. P. (2012) 1H, 13C, 15N assignment and
735
secondary structure determination of glutamine amido transferase subunit of gaunosine
736
monophosphate synthetase from Methanocaldococcus jannaschii., Biomol NMR
737
Assign.6, 193-196.
738
24.
Muchmore, D. C., McIntosh, L. P., Russell, C. B., Anderson, D. E., and Dahlquist, F. W.
739
(1989) Expression and nitrogen-15 labeling of proteins for proton and nitrogen-15
740
nuclear magnetic resonance., Methods Enzymol.177, 44-73.
741
25.
Patel, N., Moyed, H. S., and Kane, J. F. (1977) Properties of xanthosine-5'-
742
monophosphate amidotransferase from Escherichia coli., Archives of biochemistry and
743
biophysics178, 652-661.
33 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
744
26.
Moyed, H. S., and Magasanik, B. (1957) Enzymes essential for the biosynthesis of
745
nucleic acid guanine; xanthosine 5'-phosphate aminase of Aerobacter aerogenes., J Biol
746
Chem.226, 351-363.
747
27.
Mori, S., Abeygunawardana, C., Johnson, M. O., and van Zijl, P. C. (1995) Improved
748
sensitivity of HSQC spectra of exchanging protons at short interscan delays using a new
749
fast HSQC (FHSQC) detection scheme that avoids water saturation, J Magn. Reson.
750
B108, 94-98.
751
28.
Piotto, M., Saudek, V., and Sklenar, V. (1992) Gradient-tailored excitation for single-
752
quantum NMR spectroscopy of aqueous solutions, Journal of biomolecular NMR2, 661-
753
665.
754
29.
Marion, D., Driscoll, P. C., Kay, L. E., Wingfield, P. T., Bax, A., Gronenborn, A. M., and
755
Clore, G. M. (1989) Overcoming the overlap problem in the assignment of 1H NMR
756
spectra of larger proteins by use of three-dimensional heteronuclear 1H-15N Hartmann-
757
Hahn-multiple quantum coherence and nuclear Overhauser-multiple quantum coherence
758
spectroscopy: application to interleukin 1 beta., Biochemistry29, 6150 - 6156.
759
30.
Farrow, N. A., Muhandiram, R., Singer, A. U., Pascal, S. M., Kay, C. M., Gish, G.,
760
Shoelson, S. E., Pawson, T., Forman-Kay, J. D., and Kay, L. E. (1994) Backbone
761
dynamics of a free and phosphopeptide-complexed Src homology 2 domain studied by
762
15
763
31.
N NMR relaxation, Biochemistry33, 5984-6003.
Farrow, N. A., Zhang, O., Forman-Kay, J. D., and Kay, L. E. (1994) A heteronuclear
764
correlation experiment for simultaneous determination of 15N longitudinal decay and
765
chemical exchange rates of systems in slow equilibrium, J Biomol NMR.4, 727-734.
34 ACS Paragon Plus Environment
Page 34 of 66
Page 35 of 66
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
766
Biochemistry
32.
Vranken, W. F., Boucher, W., Stevens, T. J., Fogh, R. H., Pajon, A., Llinas, M., Ulrich,
767
E. L., Markley, J. L., Ionides, J., and Laue, E. D. (2005) The CCPN data model for NMR
768
spectroscopy: development of a software pipeline, Proteins59, 687-696.
769
33.
Kay, L. E., Torchia, D. A., and Bax, A. (1989) Backbone Dynamics of Proteins As
770
Studied by 15N Inverse Detected Heteronuclear NMR Spectroscopy: Application to
771
Staphylococcal Nuclease., Biochemistry28, 8972 - 8979.
772
34.
Delaglio, F., Grzesiek, S., Vuister, G. W., Zhu, G., Pfeifer, J., and Bax, A. (1995)
773
NMRPipe: a multidimensional spectral processing system based on UNIX pipes, J
774
Biomol NMR.6, 277-293.
775
35.
Shen, Y., Delaglio, F., Cornilescu, G., and Bax, A. (2009) TALOS+: a hybrid method for
776
predicting protein backbone torsion angles from NMR chemical shifts, Journal of
777
biomolecular NMR44, 213-223.
778
36.
Rev Biophys.31, 145-237.
779 780
Guntert, P. (1998) Structure calculation of biological macromolecules from NMR data, Q
37.
Guntert, P., Billeter, M., Ohlenschlager, O., Brown, L. R., and Wuthrich, K. (1998)
781
Conformational analysis of protein and nucleic acid fragments with a new grid search
782
algorithm FOUND., Journal of biomolecular NMR12, 543-548.
783
38.
analysis of macromolecular structures, J Mol Graph.14, 51-55, 29-32.
784 785
39.
788
Bhattacharya, A., Tejero, R., and Montelione, G. T. (2007) Evaluating protein structures determined by structural genomics consortia, Proteins66, 778-795.
786 787
Koradi, R., Billeter, M., and Wuthrich, K. (1996) MOLMOL: a program for display and
40.
Holm, L., and Rosenstrom, P. (2010) Dali server: conservation mapping in 3D, Nucleic Acids Res.38, W545-549. 35 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
789
41.
Schrodinger, LLC. (2010) The PyMOL Molecular Graphics System, Version 1.3r1.
790
42.
Cavanagh, J., Fairbrother, W. J., Palmer, A. G. I., Rance, M., and Skelton, N. J. (2007)
791
Protein NMR Spectroscopy: Principles and Practice, Second Edition ed., Elsevier
792
Academic Press, Amsterdam.
793
43.
constants, Curr Top Med Chem.3, 39-53.
794 795
Fielding, L. (2003) NMR methods for the determination of protein-ligand dissociation
44.
Rajagopal, P., Waygood, E. B., Reizer, J., Saier, M. H., Jr., and Klevit, R. E. (1997)
796
Demonstration of protein-protein interaction specificity by NMR chemical shift mapping,
797
Protein Sci.6, 2624-2627.
798
45.
Schmiedeskamp, M., Rajagopal, P., and Klevit, R. E. (1997) NMR chemical shift
799
perturbation mapping of DNA binding by a zinc-finger domain from the yeast
800
transcription factor ADR1, Protein Sci.6, 1835-1848.
801
46.
spectroscopy, Trends in biotechnology24, 22-27.
802 803
47.
Zuiderweg, E. R. (2002) Mapping protein-protein interactions in solution by NMR spectroscopy, Biochemistry41, 1-7.
804 805
Vaynberg, J., and Qin, J. (2006) Weak protein-protein interactions as probed by NMR
48.
Yokogawa, M., Kobashigawa, Y., Yoshida, N., Ogura, K., Harada, K., and Inagaki, F.
806
(2012) NMR Analyses of the Interaction between the FYVE Domain of Early Endosome
807
Antigen 1 (EEA1) and Phosphoinositide Embedded in a Lipid Bilayer, J. Biol. Chem.287,
808
34936-34945.
809 810
49.
Ramachandran, G. N., Ramakrishnan, C., and Sasisekharan, V. (1963) Stereochemistry of polypeptide chain configurations, J Mol Biol.7, 95-99.
36 ACS Paragon Plus Environment
Page 36 of 66
Page 37 of 66
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
811
Biochemistry
50.
proteins, Advances in protein chemistry23, 283-437.
812 813
51.
Nardini, M., and Dijkstra, B. W. (1999) Alpha/beta hydrolase fold enzymes: the family keeps growing, Curr Opin Struct Biol.9, 732-737.
814 815
Ramachandran, G. N., and Sasiskharan, V. (1968) Conformation of polypeptides and
52.
Maruoka, S., Lee, W. C., Kamo, M., Kudo, N., Nagata, K., and Tanokura, M. (2005)
816
Crystal structure of glutamine amidotransferase from Pyrococus horikoshii OT3, Proc.
817
Japan Acad.81, 459-462.
818
53.
List, F., Bocola, M., Haeger, M. C., and Sterner, R. (2012) Constitutively active
819
glutaminase variants provide insight into the activation mechanism of anthranilate
820
synthase., Biochemistry51, 2812-2818.
821
54.
List, F., Vega, M. C., Razeto, A., Hager, M. C., Sterner, R., and Wilmanns, M. (2012)
822
Catalysis uncoupling in a glutamine amidotransferase bienzyme by unblocking the
823
glutaminase active site, Chem Biol.19, 1589-1599.
824
55.
Abbott, J. L., Newell, J. M., Lightcap, C. M., Olanich, M. E., Loughlin, D. T., Weller, M.
825
A., Lam, G., Pollack, S., and Patton, W. A. (2006) The effects of removing the GAT
826
domain from E. coli GMP synthetase, The protein journal25, 483-491.
827
56.
acivicin inactivation of triad glutamine amidotransferases., Biochemistry40, 876-887.
828 829
Chittur, S. V., Klem, T. J., Shafer, C. M., and Davisson, V. J. (2001) Mechanism for
57.
Reichman, D., Cohen, M., Abramovich, R., Dym, O., Strynadka, N. C., and Schreiber, G.
830
(2007) Binding hot spots in the TEM1-BL1P interface in light of its modular architecture,
831
J Mol Biol.365, 663-679.
37 ACS Paragon Plus Environment
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1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
832
58.
Reichmann, D., Rahat, O., Albeck, S., Meged, R., Dym, O., and Schreiber, G. (2005) The
833
modular architecture of protein-protein binding interfaces, Proceedings of the National
834
Academy of Sciences of the United States of America102, 57-62.
835
59.
Swapna, L. S., Bhaskara, R. M., Sharma, J., and Srinivasan, N. (2012) Roles of residues
836
in the interface of transient protein-protein complexes before complexation., Sci Rep.2,
837
334.
838 839
60.
Sheinerman, F. B., Norel, R., and Honig, B. (2000) Electrostatic aspects of proteinprotein interactions, Curr Opin Struct Biol.10, 153-159.
840
841
842 843 844 845 846 847
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Biochemistry
848 849
Table 1
850
NOE-based distance restraints Total Intra-residue [|i-j| = 0] Sequential [|i-j| = 1] Medium range [|i-j| ≤ 4 Long range [|i-j|] ≥ 5 NOE restraints per residueb Hydrogen bond restraints Dihedral angle restraints Total number of restraintsb Total number of restraints per residueb Total number of structures calculated Number of structures used Restraint violatonsa,c Dihedral angle > 5° Distnace > 0.2 Ǻ Van der Waals Ramachandaran Plot (Procheck) Most favoured regions (%) Additionally allowed regions (%) Generously allowed regions (%) Total allowed regions (%) Disallowed regions (%) Ramachandaran Plot (Richardson’s lab) Most favoured regions (%) Allowed regions (%) Total allowed regions (%) Disallowed regions (%) rmsd from mean structure coordinate (Å) Backbonea Average heavy atoma a Analysed for residues 1 to 188
851
b
There are 183 residues with conformationally restricting restraints
852
c
Calculated for all restraints for the given residues, using average r-6
1781 670 526 200 385 9.73 110 364 2255 12.32 100 20 0 0 3 81.6 17.7 0.1 99.4 0.6 92.5 7.0 99.5 0.5 0.3 0.8
853 854 855 39 ACS Paragon Plus Environment
Biochemistry
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46 47 48 49 50 51 52 53 54 55 56 57 58 59 60
856 857
Table 2 Directly interacting residues
V12, H13, H16, R17, S18, L19, K20, Y21, I22, V24, N31 (side chain), L49, G51, G52, I55, N67 (side chain), I75, C76, L77, H79, A121, W122, A123, S124, H125, H141, C145, A149, V160, F162, H163, V166, H168, T169, E174, L176 and N178(side chain)
Indirectly interacting residues
V3, I4, D6, G23, I28, K57, I82, V90, G91, R92, A93, A95, E96, E97, Y98, A99, K102, V103, Y104, D106, D127, E128, V129, K130, Q146, E165, N173 (side chain)
858 859 860
861
862
863
864
865
866
867
868
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Biochemistry
869
870
Figure Legends
871
Figure 1:
872
and ATPPase (dimer) on a Superdex-200 column. Inset shows the molecular weight calibration
873
curve obtained using β-amylase, ADH (alcohol dehydrogenase), BSA (bovine serum albumin),
874
carbonic anhydrase and cytochrome c as the molecular weight markers.
875
Figure 2:
876
GATase subunit.
877
Figure 3:
878
HSQC spectrum of Mj GATase subunit. Strong sequential backbone HN-HN and Hα-HN NOE
879
correlations for the residues 35 to 40 indicate that these residues constitute an α-helix. Side-chain
880
to backbone NOE correlations have been also shown in figure.
881
Figure 4:
882
have been superposed on the backbone (N, Cα, and C’ atoms).
Gel filtration chromatogram showing the elution profile of Mj GATase (monomer)
Sequence specifically assigned two-dimensional 1H-15N HSQC spectrum of Mj
Two-dimensional strip-plots from the three-dimensional
15
N-edited1H-1H NOESY-
(a) Ensemble of 20 low-energy conformers of Mj GATase subunit. The structures
(b) A ribbon representation of lowest energy conformer of Mj GATase subunit.
883
884
Figure 5:
An overlay of solution NMR representative structure of Mj GATase, shown in green
885
and X-ray structure of Ph GATase(PDB ID 2D7J), shown in blue. The shortening of β-sheets
886
observed in solution structure, have been circumscribed byred elipses. Residues 68-70 and 51, 52
887
are shown in red and magenta colors respectively. The 310 helix observed in X-ray structure of
41 ACS Paragon Plus Environment
Biochemistry
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Page 42 of 66
888
Ph GATase has been circumscribed by a red circle. The catalytic residues Cys, His and Glu have
889
been shown in stick representation.
890
Figure 6:
891
values of T1(top panel) and T2(bottom panel) have been plotted as function of residue number.
892
Shown in inset in lower panel is the T2 value of C-terminus E188. The secondary structural
893
elements have been shown as cylinder (α-helix) and arrow (β-sheet).
894
Figure 7:
895
GATase + ATPPase + Q; 4 GATase + ATPPase + Mg2+ + Q + ATP; 5, GATase + ATPPase +
896
Mg2+ + Q + XMP; 6, GATase + ATPPase + Mg2+ + Q + ATP + XMP. See the text for details.
15
N T1, T2 relaxation times, measured on an Agilent 600 NMR spectrometer. The
(a) Measurement of Mj GATase activity: 1, GATase + Q; 2, ATPPase + Q; 3,
(b) GMP sythetase activity monitored by NMR. The formation of GMP is
897 898
accompanied by a concomitant decrease in the XMP concentration. See text for details.
899
Figure 8:
900
intensity of the AMP peak as a function of time is visible as the reaction progresses. Note that
901
AMP formation results from the XMP-dependent cleavage of ATP. AMP build up can be seen
902
clearly by tracking the H8 resonance of AMP.
903
Figure 9:
904
and ATPPase. Maximum activity is observed for a 1:1 ratio of GATase:ATPPase.
905
Figure 10: (a) Change in chemical shift observed in various 1H-15N HSQC spectra of
906
labeled MjA GATase subunit, upon titration with varying of MgCl2 concentration. The change in
907
chemical shift has been shown with respect to unbound protein.
Progress of the reaction independently catalyzed by Mj ATPPase subunit. Increase in
Measurement of Mj GMP synthetase activity for different stoichiometries of GATase
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15
N-
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Biochemistry
908
(b) Cartoon-surface representation of the Mg2+ binding sites on Mj GATase structure.
909
The catalytic residues are shown in red (stick representation). The residues which bind with
910
Mg2+ and are present around the catalytic site, have been shown in blue. The residues shown in
911
cyan are those showing significant chemical perturbation due to conformational changes upon
912
Mg2+ binding.
913
(c) Fitting of titration curve for some of the well resolved Mj GATase residues.
914
Figure 11: Ligand mediated association of GATase with ATPPase. (a) Elution profile of Mj
915
GATase (A) and ATPPase (B) on an analytical size-exclusion Superdex 200 column under
916
different conditions viz., 2 mM MgCl ; 2 mM MgCl + 100 µM ATP; 2 mM MgCl + 100 µM 2
917
2
2
XMP; 2 mM MgCl + 100 µM ATP + 100 µM XMP (b to e) SDS-PAGE of the the protein 2
918
fractions collected under different conditions indicated in panel by analytical gelfiltration.
919
Protein bands were developed by silver staining of the gel.
920
Figure 12: Interaction between Mj GATase and ATPPase subunits. Lane1, GATase flow through
921
(cont); lane2, GATase flow through (exp); lane 3, GATase wash (cont); lane 4, GATase wash
922
(exp); lane5, GATase + ATPPase flow through (cont.); lane 6, GATase + ATPPase flow through
923
(exp); lane 7, GATase + ATPPase wash (cont); lane 8, GATase + ATPPase wash (exp); lane 9,
924
Elute (cont); lane10 Elute (exp); lane 11 Elute fraction 2(cont); lane 12 Elute fraction 2 (exp);
925
lane 13 beads (cont); lane 14 beads (exp); M is the molecular weight marker. Note (exp) refers
926
to experiment done in presence of ligands, while (cont.) is that in the absence of ligands.
927
Experimental details are as described in methods.
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928
Figure 13: (a) Overlay of proton one dimensional spectra of GATase, ATPPase and GATase,
929
ATPPase in presence of all substrates. The observed line broadening has been highlighted in red
930
rectangles.
931
(b) Overlay of two-dimensional 1H-15N spectra of
15
N-labeled Mj GATase subunit.
932
The red and blue colored spectra represent the spectra of GATase in absence and presence of
933
ATPPase subunit, respectively. Both of the spectra were acquired in absence of substrates.
934
(c) Overlay of two-dimensional 1H-15N spectra of
15
N-labeled Mj GATase subunit.
935
The spectrum shown in red represents the GATase spectrum in presence of unbound ATPPase
936
subunit. The blue spectrum represents the GATase spectrum in presence of ligand bound
937
ATPPase. Shown in inset is decrease in intensity upon GATase-ATPPase interaction.
938
(d) Decrease in intensity of 1H-15N correlation peaks of 15N-labeled GATase subunit
939
as a function of ATPPase concentration. All spectra were acquired in presence of the constant
940
saturating concentration of substrates. See text for details.
941
Figure 14: (a) Plot of normalized change in intensity as a function of residue number of Mj
942
GATase subunit. The residues showing ∆Inormalized> 0.80 and ∆Inormalized ≥0.75≤ 0.80 are shown in
943
blue and cyan, respectively. The catalytic residues are shown in red.
944
(b) Cartoon representation of Mj GATase subunit showing ATPPase interaction sites.
945
The catalytic residues have been shown in red (stick representation). The residues involved in
946
direct interaction are shown in blue while those involved in indirect interaction are shown in
947
cyan. The positively charged α-helix is highlighted in red elipse.
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Biochemistry
(c) Surface representation of Mj GATase subunit, showing the interaction surface
948 949
between two subunits.
950
Figure 15: Surface potential representation of Mj GATase structure. Large negatively charge
951
patches can be seen on both sides of the Mj GATase structure.
952
Figure 1
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Biochemistry
Figure 2
977 978 979 980 981 982
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Figure 3
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Biochemistry
Figure 4a
988 989 990 991 992 993 994 995 996 997 998 999 1000 1001 1002 1003 1004 1005 1006 1007 1008 1009 1010
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Figure 4b
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Biochemistry
Figure 5
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1045
Figure 6
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Biochemistry
Figure 7a
1051 1052 1053 1054 1055 1056 1057 1058 1059
Figure 7b
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1062
Figure 8
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Biochemistry
Figure 9
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Figure 10a
1085 1086 1087 1088 1089 1090 1091 1092 1093
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Biochemistry
Figure 10b
1095
1096 1097
Figure 10c
1098 1099 1100 1101
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1102
Figure 11 (a)
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Biochemistry
Figure 12
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Biochemistry
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1125
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Figure 13a
1126 1127 1128
Figure 13b
Figure 13c
1129
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Biochemistry
Figure 13d
1131
1132 1133 1134 1135 1136 1137 1138 1139 1140 1141 1142 1143 1144 1145
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Figure 14a
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Biochemistry
Figure 14b
1171 1172 1173 1174 1175 1176 1177 1178 1179 1180 1181 1182 1183 1184 1185
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Figure 14c
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Biochemistry
Figure 15
1201 1202 1203 1204 1205 1206 1207 1208 1209 1210 1211 1212 1213 1214 1215
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1216
For Table of Contents Use Only
1217
Solution NMR structure of GATase subunit and structural basis of interaction between GATase
1218
and ATPPase subunits in a two-subunit-type GMPS from Methanocaldococcus jannaschii
1219
Rustam Ali, Sanjeev Kumar, Hemalatha Balaram and Siddhartha P. Sarma
1220
1221
1222
1223
1224
1225
1226
1227
1228
1229
1230
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