Competitive Upconversion-Linked Immunosorbent Assay for the

Photon-upconverting nanoparticles (UCNPs) emit light of shorter wavelength under near-infrared excitation and thus avoid optical background interferen...
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A competitive Upconversion-Linked Immunosorbent Assay (ULISA) for the rapid and sensitive detection of diclofenac Antonín Hlavá#ek, Zden#k Farka, Maria Hübner, Veronika Hor#áková, Daniel Nemecek, Reinhard Niessner, Petr Skládal, Dietmar Knopp, and Hans H Gorris Anal. Chem., Just Accepted Manuscript • DOI: 10.1021/acs.analchem.6b01083 • Publication Date (Web): 11 May 2016 Downloaded from http://pubs.acs.org on May 12, 2016

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Analytical Chemistry

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A competitive Upconversion-Linked Immunosorbent Assay

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(ULISA) for the rapid and sensitive detection of diclofenac

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Antonín Hlaváček†,‡,§, Zdeněk Farka†,‡, Maria Hübnerǁ, Veronika Horňáková‡, Daniel

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Němeček‡, Reinhard Niessnerǁ, Petr Skládal‡, Dietmar Knoppǁ, Hans H. Gorris†*

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Institute of Analytical Chemistry, Chemo- and Biosensors, University of Regensburg, 93040 Regensburg, Germany ‡

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CEITEC - Central European Institute of Technology, Masaryk University, Brno 625 00, Czech Republic

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§

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ǁ

Institute of Analytical Chemistry AS CR, v. v. i., Brno 602 00, Czech Republic

Chair for Analytical Chemistry and Institute of Hydrochemistry, Technical University of Munich, 81377 Munich, Germany

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*Corresponding author

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Hans H. Gorris, PhD

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Institute of Analytical Chemistry, Chemo- and Biosensors University of Regensburg Universitätsstr. 31 93040 Regensburg

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Germany

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Tel.: +49-941-943-4015

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Fax: +49-941-943-4064

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e-mail: [email protected]

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Abstract

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Photon-upconverting nanoparticles (UCNPs) emit light of shorter wavelength under near-

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infrared excitation and thus avoid optical background interference. We have exploited this

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unique photophysical feature to establish a sensitive competitive immunoassay for the

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detection of the pharmaceutical micropollutant diclofenac (DCF) in water. The so-called

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upconversion-linked immunosorbent assay (ULISA) was critically dependent on the design of

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the upconversion luminescent detection label. Silica-coated UCNPs (50 nm in diameter)

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exposing carboxyl groups on the surface were conjugated to a secondary anti-IgG antibody.

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We investigated the structure and monodispersity of the nanoconjugates in detail. Using a

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highly affine anti-DCF primary antibody, the optimized ULISA reached a detection limit of

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0.05 ng DCF per mL. This performance comes close to a conventional ELISA without the

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need for an enzyme-mediated signal amplification step. The ULISA was further employed for

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analyzing drinking and surface water samples and the results were consistent with a

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conventional ELISA as well as LC-MS.

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Introduction

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The enzyme-linked immunosorbent assay (ELISA) is a cost efficient tool for the specific and

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highly sensitive detection of many toxic analytes in food and environmental samples as well

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as clinical diagnosis. There are, however, some disadvantages of a classic ELISA such as an

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inherent instability of enzymes and time consuming signal development. Consequently, many

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research efforts have been made to replace the enzymes by using nanoparticles (NPs) as

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signal amplifiers, e.g. fluorescent dye-doped polymer or silica NPs,1 metal NPs,2 magnetic

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NPs,3

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(UCNPs) have been used as a new generation of luminescent labels for sensitive

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immunochemical detection. UCNPs are lanthanide-doped nanocrystals that can be excited by

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near-infrared light and emit light of shorter wavelengths (anti-Stokes emission),6,7 which

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strongly reduces autofluorescence and light scattering. Further advantages of UCNPs include

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(A) a very high photostability, (B) large anti-Stokes shifts allowing for an excellent separation

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of excitation and detection channels, and (C) multiple and narrow emission bands that can be

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tuned individually for the multiplexed detection of analytes.8-10

catalytic NPs4 or quantum dots.5 Recently, photon-upconverting nanoparticles

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These distinct photophysical features of UCNPs have been used for the design of

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heterogeneous microtiter plate immunoassays, e.g. for the detection of prostate-specific 2 ACS Paragon Plus Environment

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antigen (limit of detection, LOD: 0.15 ng mL-1 / 6 pM)11 or human chorionic gonadotropin

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(LOD: 3.8 ng mL-1 / 200 pM).12 The advantages of UCNPs in lateral flow assays e.g. for the

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detection of worm parasite antigens (LOD: 0.01 ng mL-1 / 0.1 pM)13 have also been well

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documented. There have been a few reports on the use of homogeneous competitive

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immunoassays for the detection of small molecules such as estradiol (LOD: ~0.1 ng mL-1 /

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400 pM)14 and folate (LOD: 0.4 ng mL-1 / 1000 pM)15 in blood and a bead-based

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immunoassay for the detection of mycotoxins in food samples (LOD: ~0.01 ng mL-1 / 50

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pM).16

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The development and widespread availability of more sensitive analytical techniques has

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resulted in an increasing number of pharmaceuticals that can be detected in the environment

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after medical or veterinary use.17,18 Diclofenac (2-[2-(2,6-dichlorophenyl) aminophenyl]

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ethanoic acid; DCF) is a widely used non-steroidal anti-inflammatory drug (NSAID). In the

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Indian subcontinent, the widespread use of DCF for veterinary treatment of cattle since the

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1990s has led to a precipitous decline of the indigenous vulture population because DCF leads

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to renal failure in vultures that feed on contaminated carcasses.19 In Europe, DCF belongs to

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the most frequently detected pharmaceuticals in the water-cycle because it is not easily

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degraded when passing through sewage treatment plants. DCF has been detected in low µg

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L−1 amounts in wastewater effluents and also in ng L-1 amounts in surface waters,20

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groundwater and drinking water.21 Very low amounts of DCF can be detected by LC-TOF-

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MS or high resolution mass spectrometers.22,23 These instrumental techniques, however, are

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expensive, time consuming, labor intensive and need trained personnel. By contrast,

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immunoassays are more suitable for on-site testing directly in the field or for the analysis of

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large numbers of samples in small laboratories.24

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Here, we have optimized the preparation of monodisperse and stable upconversion

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reporters for the sensitive detection of DCF in water samples by a competitive upconversion-

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linked immunosorbent assay (ULISA). Anti-mouse IgG antibodies were conjugated to silica-

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coated UCNPs exposing carboxyl function on the surface and the conjugates were

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characterized by gel electrophoresis.25 The competitive detection of DCF was performed

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using a monoclonal mouse anti-DCF antibody (Figure 1). This antibody was characterized in

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detail as described recently26 and showed about 10 % cross-reactivity with DCF metabolites

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such as 5-OH-DCF, 4’-OH-DCF and DCF-acyl glucuronide, but only less than 1 % with other

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structurally related non-steroidal anti-inflammatory drugs. The performance of the optimized

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ULISA was compared with a conventional ELISA as well as LC-MS. 3 ACS Paragon Plus Environment

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Figure 1. Scheme of the indirect competitive ULISA for the detection of diclofenac (DCF). (A) A microtiter plate is coated with a bovine serum albumin-DCF conjugate (BSA-DCF). (B) Dilution series of DCF are prepared in the microtiter plate followed by the addition of anti-diclofenac mouse antibody. (C) The attachment of anti-diclofenac antibody is then detected by an anti-mouse IgG-UCNP secondary antibody conjugate. The upconversion luminescence is recorded under 980 nm laser excitation.

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Experimental section

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Chemicals

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All standard chemicals and diclofenac sodium salt (D6899, purity ≥98 %) were obtained from

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Sigma-Aldrich (Steinheim, Germany). Carboxyethylsilanetriol sodium salt; 25% (w/v) in

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water was obtained from ABCR GmbH (Karlsruhe, Germany). The horseradish peroxidase-

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labeled horse anti-mouse IgG was from Axxora (Lörrach, Germany) and horse anti-mouse

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IgG was from Vector Laboratories (Burlingame, USA). The monoclonal anti-diclofenac

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antibody 12G5 was generated in mice using a DCF-thyroglobulin conjugate as described

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previously.26 An antibody stock solution of 0.45 mg mL-1 was prepared in 20 mM NaH2PO4,

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20 mM NaH2PO4, 0.1 M Tris-HCl, 0.02% NaN3, pH 7.4 and stored at 4° C. Buffers and

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solutions were prepared with ultrapure water, which was obtained by reverse osmosis with

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UV treatment (Milli-RO 5 Plus, Milli-Q185 Plus, Eschborn, Germany).

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Synthesis of carboxyl-silica-coated UCNPs

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UCNPs of 42.5 ± 4.9 nm in diameter were synthesized by high-temperature co-precipitation27

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as described in the Supporting Information. The mass concentration was determined by

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gravimetric analysis and a concentration of 1.0 mg mL-1 of UCNPs was estimated to be

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equivalent to the molar concentration of 9.8×10-9 mol L-1 (Supporting Information).

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Carboxyl-silica-coated

UCNPs

(COOH-UCNPs)

were

prepared

by

a

reverse

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microemulsion method:25 UCNPs (80 mg) were diluted in cyclohexane to a final volume of

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23 mL. This dispersion was mixed with 1800 mg of Igepal CO-520 and 100 µL of tetraethyl

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orthosilicate (TEOS) and stirred intensively for 10 min. A mixture of 55 µL 25 % (w/v)

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aqueous ammonium hydroxide and 55 µL water was added to form a microemulsion that was 4 ACS Paragon Plus Environment

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slowly stirred overnight. Then, 25 µL of TEOS were added and the microemulsion was again

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stirred for 180 min. After adding 50 µL of 25% (w/v) sodium carboxyethylsilanetriol in water,

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the microemulsion was first sonicated for 15 min and then stirred for 60 min. The COOH-

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UCNPs were extracted with 1000 µL of dimethylformamide and washed four times with 20

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mL of propan-2-ol, three times with 5000 µL of water and finally dispersed in water to yield a

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final concentration of 150 mg mL-1. The COOH-UCNPs in water were stable at 4°C for

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several months.

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Conjugation of COOH-UCNP and secondary antibody

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COOH-UCNPs were first activated by 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide

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(EDC) and N-hydroxysulfosuccinimide (sulfo-NHS). In a typical synthesis, 0.5 mg (~5 pmol)

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of COOH-UCNPs was dispersed in water to a final volume of 200 µL. The volume of 50 µL

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of a mixture containing 2.1 µmol of EDC and 5.5 µmol of sulfo-NHS in 100 µL of 100 mM

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sodium 2-(N-morpholino)ethanesulfonate (MES) buffer, pH 6.1 was added and mixed for 30

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min. A dispersion of 100 µL activated COOH-UCNPs (1 mg mL-1 or ~10 nmol L-1) were

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mixed with 100 µL of horse anti-mouse IgG in borate buffer (100 mM sodium borate, pH

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9.0). Three IgG concentrations were employed and incubated for 90 min at room temperature:

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1) 330 nmol L-1 IgG resulting in a ratio 33 IgG molecules per UCNP (sample IgG-UCNP-

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33:1). 2) 67 nmol L-1 IgG resulting in a ratio of 7 IgG molecules per UCNP (IgG-UCNP-7:1),

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and 3) 33 nmol L-1 IgG resulting in a ratio of 3 IgG molecules per UCNP (IgG-UCNP-3:1).

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The bioconjugates were centrifuged for 10 min at 4,000 g, dispersed in UCNP assay buffer

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(50 mM Tris, 150 mM NaCl, 0.05% NaN3, 0.01% Tween 20, 0.05% bovine γ-globulin

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(BGG), 0.5% bovine serum albumin (BSA), 0.2% polyvinyl alcohol 6000 (PVA), pH 7.75)

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and sonicated for 5 min.

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Nanoparticle characterization

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Transmission electron microscopy (TEM) was performed on a Tecnai F20 FEI instrument

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(Eindhoven, The Netherlands). About 4 µL of UCNPs were deposited on a 400-mesh copper

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EM grid coated with a continuous carbon layer and negatively stained with 2% (w/v) aqueous

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solution of uranyl acetate to increase the contrast of the silica shell. The dried grids were then

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imaged at 50,000× magnification (2.21 Å pixel-1). The size of individual particles in the TEM

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images was measured by the imaging software ImageJ (http://imagej.nih.gov).28 The

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hydrodynamic diameter and zeta potential of UCNP suspensions were determined on a

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Zetasizer Nano SZ from Malvern Instruments (Malvern, UK). FT-IR spectra were recorded

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on an Alpha FTIR Spectrometer from Bruker (Billerica, USA). 5 ACS Paragon Plus Environment

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Agarose gel electrophoresis

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Following our previous work,25 COOH-UCNPs and their bioconjugates were characterized by

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agarose gel electrophoresis (0.5% w/v agarose, 45 mM Tris, 45 mM H3BO3 with pH 8.6, 15

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min at 100 V). Samples were mixed in a ratio of 10:1 with 50 % w/w glycerol and 8 µL

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aliquots were loaded onto the gel. A custom-built upconversion reader (CHAMELEON

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multilabel microplate reader, Hidex, Turku, Finland) equipped with a continuous 980 nm laser

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(4 W) was used to scan agarose gels with a spatial resolution of 0.5 mm as described earlier.29

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Conjugation of diclofenac to BSA

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BSA-DCF conjugates were prepared using either 1.5 µmol or 7.5 µmol DCF and 9.7 µmol

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sulfo-NHS added to a mixture of 400 µL MES buffer and 100 µL dimethylformamide. DCF

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was activated by the addition of 47 µmol of EDC and incubation at room temperature for 30

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min. After adding 500 µL of 0.15 µmol BSA in water and 250 µL of 50 mM aqueous Na2CO3,

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the mixture was incubated at room temperature for 4 hours and then dialyzed three times

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against 150 mL of 50 mM Na2CO3. BSA-DCF was adjusted to a concentration of 1.6 mg

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mL−1 by adding 50 mM of Na2CO3 and stored at 4 °C in presence of 0.05 % NaN3. The

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conjugate was analyzed by MALDI-TOF-MS (Bruker, Ultraflex TOF/TOF, N2-laser, 337 nm,

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positive mode).

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Water samples

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Munich tap water and two surface water samples were collected in Southern Bavaria from

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lake Wörthsee and river Würm. The fresh water samples were filtrated over a glass microfiber

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filter (GF/C, Whatman Cat. No. 1822 047) and stored at 4°C. The concentrations of Ca2+,

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Mg2+, and dissolved organic content (DOC) as well as the conductivity and pH were

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determined (Supporting Information Table 1). ELISA and ULISA were performed with

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undiluted and spiked samples. For LC-MS, the samples were subjected to generic solid phase

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extraction (SPE) and analyzed by an Orbitrap-based ExactiveTM Benchtop Mass Spectrometer

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(Thermo Scientific, Dreieich, Germany) as described earlier26.

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Upconversion-linked immunosorbent assay (ULISA)

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A transparent 96-well microtiter plate with high protein binding capacity (Corning,

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Wiesbaden, Germany) was coated with BSA-DCF in coating buffer (optimal concentration: 1

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µg mL-1 BSA-DCF in 50 mM NaHCO3 /Na2CO3, 0.05% NaN3, pH 9.6; 200 µL per well) at

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4° C over night. All subsequent steps were carried out at room temperature. The plate was

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washed manually four times with 250 µL of washing buffer (50 mM Na/H2PO4/HPO4, 0.01% 6 ACS Paragon Plus Environment

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Tween 20, 0.05% NaN3, pH 7.4). The free binding sites in each well were blocked with 250

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µL of 1% BSA in 50 mM Na/H2PO4/HPO4, 0.05 % NaN3, pH 7.4 for 1 h. The plate was

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washed four times with washing buffer. Either standard dilutions of DCF in double distilled

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water or environmental samples (100 µL per well) were added, immediately followed by the

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anti-DCF monoclonal mouse antibody (12G5, optimal concentration: 0.225 µg mL−1 in 100

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mM NaPO4, 300 mM NaCl, 100 µL per well) and incubated for 1 h. After four washing steps,

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the microtiter plate was incubated for one hour with 100 µL of the IgG-UCNP conjugate

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(optimal concentration: 10 µg mL−1 in 50 mM Tris, 150 mM NaCl, 0.05% NaN3, 0.01%

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Tween 20, 0.05% BGG, 0.5% BSA, 0.2% PVA, pH 7.75). After four washing steps, the

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upconversion luminescence was read out from empty wells using a custom-built upconversion

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microplate reader (CHAMELEON multilabel microplate reader, Hidex, Turku, Finland)

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equipped with a continuous 980 nm laser (4 W). A collimated laser spot of ~0.8 mm was

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focused on the bottom of the microtiter wells. Each well was scanned 100 times in a raster

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with the step size of 0.4 mm and 500 ms signal integration time. The truncated mean was

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calculated for each well after discarding the ten highest and ten lowest measurements of the

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luminescence intensity to account for local irregularities on the microtiter well surface that

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result in signal outliers.

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Enzyme-linked immunosorbent assay (ELISA)

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The ELISA was performed as described earlier.26 A transparent 96-well microtiter plate with

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high protein binding capacity (Greiner Bio-one, Frickenhausen, Germany) was coated with

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0.5 µg mL−1 of ovalbumin-DCF conjugate in coating buffer (50 mM NaHCO3/Na2CO3, 0.05%

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NaN3, pH 9.6; 200 µL per well) at 4 °C over night. All subsequent steps were carried out at

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room temperature. The plate was automatically washed with a plate washer (ELx405 Select,

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Bio-Tek Instruments, Bad Friedrichshall, Germany) four times with washing buffer (50 mM

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K/H2PO4/HPO4, 146 mM NaCl, 0.05% Tween 20, pH 7.6; PBST). The free binding sites in

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each well were blocked with 300 µL of 1% BSA in PBST for 1 h. The plate was washed four

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times with washing buffer. First, standard dilutions of DCF in double distilled water or

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environmental samples (100 µL per well) were added, immediately followed by the anti-DCF

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monoclonal mouse antibody (12G5, 0.5 µg mL−1 in PBS; 100 µL per well) and incubated for

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30 min. After four washing steps, the secondary horseradish peroxidase-labeled antibody was

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added (0.2 mg mL-1 in PBS; 200 µL per well) and incubated for 1 h. After final washing, the

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substrate solution (200 µL per well) was added and the plates were shaken for about 15 min

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for color development. The substrate solution consisted of 25 mL substrate buffer (prepared 7 ACS Paragon Plus Environment

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with 46.0 mL potassium dihydrogen citrate and 0.1 g potassium sorbate in 1 L of water, pH

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3.8), 500 µL 3,3',5,5'-tetramethylbenzidine stock solution (375 mg in 30 mL of

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dimethylsulfoxide) and 100 µL 1% hydrogen peroxide. The enzyme reaction was stopped by

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adding 100 µL of 5% sulfuric acid per well. The absorbance was read at 450 nm by a

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microplate reader (Synergy HT, Bio-Tek Instruments).

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Data analysis

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A four-parameter logistic function (Eq. 1) was used for a regression analysis of the calibration

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curves:

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Y =

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where [DCF] is the concentration of diclofenac, and Y is either the upconversion

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luminescence or the absorbance at 450 nm. Eq. 1 yields the maximum (Ymax) and background

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(Ybg) signal, the DCF concentration that reduces (Ymax-Ybg) by 50 % (IC50) and the slope at the

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inflection point (s). All measurements were made at least in triplicate. The concentration of

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DCF in real water samples was determined by utilizing an inverse function of Eq. 1 and the

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limit of detection (LOD) was defined as before:26

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Y(LOD) = 0.85 × (Ymax - Ybg) + Ybg

Ymax − Ybg  [ DCF ]   1 +   IC 50 

s

+ Ybg

(1)

(2)

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Results and Discussion

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Surface modification and characterization of UCNPs

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The development of a competitive upconversion immunoassay (ULISA) for the detection of

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DCF (Figure 1) critically depends on the design of the luminescent reporter that replaces the

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conventional enzyme amplification steps.30 Oleic acid-capped UCNPs were coated with a

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silica shell exposing carboxylic acid functional groups on the surface. The carboxyl groups

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improve the dispersibility in water and serve as attachment sites for subsequent conjugation

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steps. We previously described a one-step water-in-oil microemulsion protocol for coating the

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surface of small UCNPs (~12 nm in diameter) with a carboxylated silica shell that showed

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only a weak upconversion luminescence.25 For the immunoassay, we have synthesized larger

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UCNPs of 42.5 ± 4.9 nm in diameter (Supporting Information Figure S1) that are much

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brighter because they are less affected by surface quenching effects.31 The one step silica8 ACS Paragon Plus Environment

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coating protocol, however, resulted in aggregation when directly applied to bigger

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nanoparticles. Therefore, we developed a two-step protocol to prepare a thicker, compact and

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more stable silica shell on the surface of UCNPs.32 First, TEOS was added to the

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microemulsion to generate a thin layer of bare silica (2.4 ± 0.4 nm, Supporting Information

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Figure S2). This step alone was not sufficient to prevent aggregation. Therefore, TEOS was

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added for a second time, which changed the thickness of the silica shell only slightly. The

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second carboxylation step ensured an excellent dispersibility of COOH-UCNP in water.33 The

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total diameter of COOH-UCNPs was consistent as determined by transmission electron

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microscopy (TEM: 46.9 ± 5.0 nm; Supporting Information Figure S3 and Figure 2A) and

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atomic force microscopy (AFM: 45.4 ± 7.6 nm; Supporting Information Figure S4). Dynamic

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light scattering measurements confirmed an increase of the hydrodynamic diameter from 55

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nm to 65 nm after silica coating (Supporting Information Figure S5).

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The optimized COOH-UCNPs were then conjugated to a secondary anti-IgG antibody via

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standard EDC/sulfo-NHS chemistry (Figure 2B).34,35 A low concentration of COOH-UCNP

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was utilized to prevent that one antibody molecule binds to several UCNPs, which would lead

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to aggregation. The conjugates were characterized by agarose gel electrophoresis (Figure 2C),

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dynamic light scattering (DLS), zeta potential measurements and FT-IR spectroscopy

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(Supporting Information Figures S6-S8). The lowest degree of aggregation was observed

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when the concentration of COOH-UCNPs in the reaction mixture was 1 mg mL-1. The

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conjugation of the secondary antibody reduced the negative surface potential of the COOH-

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UCNPs as shown by zeta potential measurements and led to a stronger retardation in the

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agarose gel.36 The shift of the electrophoretic mobility was linearly dependent on the ratio of

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IgG molecules per UCNP and indicated the degree of surface modification (Figure 2D).

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Additionally, larger aggregates of nanoparticles remained in the gel pockets and could not

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enter the agarose matrix. Sample IgG-UCNP-33:1 shows a main fraction of monodisperse

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bioconjugates separated as a distinct band and a smaller fraction of slowly moving

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components, which are probably partially aggregated and crosslinked bioconjugates. This

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result is consistent with a bimodal particle distribution and a higher polydispersity index

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observed in the DLS measurement.

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The IgG-UCNP conjugates were purified from an excess of unbound secondary anti-mouse

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IgG and components of the reaction mixture by differential centrifugation. At first, the

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bioconjugates were centrifuged at 10,000 g, which, however, led to strong nanoparticle

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aggregation (Figure 2C). When the centrifugal speed was reduced to 4,000 g followed by 9 ACS Paragon Plus Environment

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short sonication, purified and monodisperse IgG-UCNP were obtained. Further lowering of

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the centrifugal field was not efficient since the sedimentation of IgG-UCNP was too slow.

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The small retardation coefficient of UCNPs prepared with the lowest amount of IgG (IgG-

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UCNP-3:1, Figure 2C, lane V) indicated an insufficient surface modification. Therefore, this

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bioconjugate was not used for the following ULISA experiments.

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292 293 294 295 296 297 298 299 300 301

Figure 2. Preparation and characterization of IgG-UCNP conjugates. (A) TEM image of silica-coated UCNPs exposing carboxyl groups on the surface (COOH-UCNPs, Supporting Information Figure S3). (B) The carboxyl groups are activated by EDC/sulfo-NHS and conjugated to anti-mouse IgG. (C) The conjugates are prepared by using different ratios of anti-mouse IgG and COOH-UCNPs (I/II: 33 to 1; III/IV: 7 to 1; V/VI: 3 to 1, VII/VIII: no IgG). Each sample is centrifuged either with 4,000 g (I, III, V, VII) or with 10,000 g (II, IV, VI, VIII) and characterized by agarose gel electrophoresis. The migration distance (∆) is indicated with red lines. (D) The relative electrophoretic mobility (∆ratio[x]/∆no IgG) of the conjugates is linearly dependent on the ratio of IgG molecules per UCNP.

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Design of Upconversion-linked immunosorbent assay (ULISA)

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In a competitive immunoassay, a low concentration of coating antigen ensures that the free

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analyte can compete efficiently for the binding sites of the detection antibodies. On the other

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hand, the signal generation has to be strong enough for a reliable readout. Here, we prepared

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two different coating conjugates consisting of BSA-DCF. The conjugates were analyzed by

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MALDI-TOF mass spectrometry, which showed a coupling density of either 5.7 or 10 DCF

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residues per BSA molecule (Supporting Information Figures S9-S11). When the conjugate 10 ACS Paragon Plus Environment

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with the higher degree of derivatization was used for coating in the immunoassay, the signals

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were – as expected – about twice as high but also showed stronger signal fluctuation and a

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hook effect (Figure 3A), which may be the consequence of two binding sites of IgG

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molecules forming cyclic complexes (Supporting Information Figure S12).37 By contrast, the

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conjugate exposing 5.7 DCF residues per BSA molecule yielded more stable signals and a

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slightly lower IC50 value (1.2 ng mL-1 compared to 1.5 ng mL-1) and a lower detection limit

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for DCF. Consequently, this coating conjugate was used in all further experiments. An

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optimal signal generation was observed with a coating concentration of 1 µg mL-1

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(Supporting Information Figure S13).

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Figure 3. ULISA optimization. (A) Microtiter plates are coated with 1 µg mL-1 of BSA carrying either 10 (□) or 5.7 (○) DCF residues. (B) The upconversion luminescent (UCL) signal is generated by using 10 µg mL-1 of IgGUCNP-33:1 (○) or IgG-UCNP-7:1 (□), respectively. (C) The detection of DCF is optimized by using the monoclonal anti-DCF antibody in concentrations of 0.5 µg mL-1 (○) (IC50: 0.68 ng mL-1), 0.25 µg mL-1 (□) (IC50: 0.23 ng mL-1), 0.1 µg mL-1 (∆) (IC50: 0.13 ng mL-1) or 0.02 (◊) µg mL-1 (IC50: 0.08 ng mL-1). Error bars represent standard deviations in upconversion signals from three replicate wells.

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The competition step including free DCF and anti-DCF detection antibody was performed

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in analogy to a sensitive conventional ELISA.26 Only the enzyme-mediated color generation

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was replaced by an IgG-UCNP conjugate as a direct luminescent reporter (Figure 3B). The

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higher degree of UCNP surface coverage (IgG-UCNP ratio of 33:1 compared to 7:1)

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increased the maximum signal intensity by a factor of five although both conjugates were

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prepared with a molar excess of IgG molecules per nanoparticle. This difference can be

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explained because not every surface-conjugated antibody may have the right orientation or be

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fully functional in order to bind efficiently to the primary antibody. Consequently, a higher

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degree of derivatization resulted in a proportionally higher number of functional antibodies.

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On the downside, using IgG-UCNP-33:1 resulted in strong signal fluctuations as well as a

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hook effect, which impedes the reproducible determination of DCF. It should also be noted

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that the degree of surface substitution did not significantly affect IC50 or the LOD, and a

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concentration of 10 µg mL-1 IgG-UCNP-7:1 resulted in the most reproducible upconversion

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signal generation (Supporting Information Figure S14)

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In contrast to the UCNP-bound secondary antibody, the primary anti-DCF antibody is

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directly involved in the competition step. Figure 3C shows that both the upconversion signal

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intensity and the IC50/LOD for DCF strongly depend on the antibody concentration. A higher

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primary antibody concentration leads to a higher signal intensity because more antibodies can

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bind to the DCF-BSA coating conjugate, but they also consume a larger amount of free DCF

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and thus deteriorate the assay sensitivity. A concentration of 0.25 µg mL-1 primary anti-DCF

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antibody yielded an optimal balance between signal generation and sensitivity for the

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determination of DCF and was used in all further experiments.

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Calibration and sensitivity of ULISA and ELISA

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For each type of competitive immunoassay it is necessary to find the optimal balance between

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detection sensitivity for an analyte and signal development. It should also be noted that a high

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affinity and a low cross-reactivity of the primary antibody are the most distinctive features

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that determine the sensitivity and specificity of the analyte detection. Figure 4 shows

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calibration curves of ULISA and ELISA recorded under similar conditions and using the same

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anti-DCF primary antibody. In both cases a signal to background ratio (Ymax/Ybg) of 5:1 was

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adjusted to achieve the most sensitive detection of DCF but also to obtain a reliable signal

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generation. The competitive ULISA (LOD: 0.05 ng mL−1 / 170 pM) has a five times higher

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detection limit than a conventional ELISA (LOD: 0.01 ng mL−1/ 34 pM) but allows for an

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easier and faster signal generation. As the detection sensitivity is ultimately dependent on the

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anti-DCF antibody, it can be expected that the ULISA can be further optimized by developing

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brighter UCNPs reporter conjugates.

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Competitive immunoassays for small molecules are typically less sensitive than sandwich

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immunoassays where the signal generation is directly proportional to the analyte

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concentration. The highest sensitivity was described for the detection of Schistosoma

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circulating anodic antigen by using micron-sized upconversion particles in a lateral flow assay

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(LOD: 0.01 ng mL-1 / 0.1 pM).13 This particular analyte displays repetitive surface epitopes

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and facilitates binding of several primary antibodies per analyte molecule. The competitive

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immunoassay for DCF affords a similar sensitivity as a magnetic bead-based competitive

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immunoassay for the detection of aflatoxin that was reported to reach an LOD of 0.01 ng mL-1

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(50 pM) under optimal conditions.16 The additional magnetic separation step, however,

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demands a more sophisticated instrumentation and is more time consuming. 12 ACS Paragon Plus Environment

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Figure 4. Normalized calibration curves of ULISA (□, replotted red curve from Figure 3C; IC50: 0.23 ng mL−1, LOD: 0.05 ng mL−1) and ELISA (○, IC50: 0.05 ng mL−1, LOD: 0.01 ng mL−1). Error bars represent standard deviations of three replicate wells.

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Detection of diclofenac in real water samples

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Two surface water samples and drinking water were collected in Southern Bavaria and the

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matrix was analyzed (Supporting Information Table S1) to assess possible interferences with

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the detection of DCF. These interferences should be as low as possible because matrix effects

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can suppress the immunoassay signal and lead to an overestimation of analyte concentrations.

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The monoclonal primary antibody 12G5 is resistant to matrix interferences over a wide pH

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range, humic acid concentrations up 20 mg L-1 and Ca2+ concentrations up to 75 mg L-1 as

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described earlier.26 The drinking water sample from Munich, however, contained relatively

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high Ca2+ and Mg2+ concentrations of 110 mg L-1 in total, which is probably the reason for a

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signal suppression (defined as 100 × (Ysample - Ybg) / (Ymax - Ybg)) to 60±7 % in the ULISA and

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73±10 % in the ELISA in the undiluted samples without DCF. By contrast, the surface water

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samples contained less Ca2+ and Mg2+ and were less affected by signal suppression.

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The concentration of DCF was too low to be detectable in the unspiked water samples.

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Thus, each sample was additionally spiked with either 1 ng mL-1 or 10 ng mL-1 of DCF. The

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spiked samples were typically diluted at least by a factor of three prior to the immunoassay to

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keep matrix effects to a minimum. Table 1 shows the concentrations of DCF as determined by

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ULISA, ELISA and LC-MS. The ULISA led to slightly stronger deviations from the spiking

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concentration compared to the ELISA because the matrix may also have an impact on the

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binding of the nanoparticulate luminescent reporter unit, which is relatively large compared to

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the enzyme antibody conjugate used for the ELISA. These differences in the immunoassay

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performance are subject to further investigation and will be optimized to unfold the full

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potential of the ULISA for the background-free detection of analytes.

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Table 1. Detection of DCF in unspiked and spiked real water samples. Sample

Lake Wörthsee

River Würm

Munich tap water

Spiked (ng mL-1)

ULISA (ng mL-1)

ELISA (ng mL-1)

LC-MS (ng mL-1)

-