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Letter NC
BNA gapmers revert splicing and reduce RNA foci with low toxicity in myotonic dystrophy cells Kassie S. Manning, Ashish N. Rao, Miguel Castro, and Thomas A. Cooper ACS Chem. Biol., Just Accepted Manuscript • DOI: 10.1021/acschembio.7b00416 • Publication Date (Web): 30 Aug 2017 Downloaded from http://pubs.acs.org on September 3, 2017
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CTG(300) GFP CMV
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A M C oc A k A NC G g ap C m A LN e G ga r A BN CA pm A NC G m er ix C AG me m r ix m er
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n.s. (p=0.15)
Control 30nM gapmer 30nM mixmer
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200000
100000 0
CNPY3
GAPDH GAPDH
1.2 1.0 0.8 0.6 0.4 0.2 0.0 ***
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B Polymorphic BpmI site
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Allele 1 DMPK allele 1 expression
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BNANC gapmers revert splicing and reduce RNA foci with low toxicity in myotonic dystrophy cells Kassie S. Manning
1, 2
3
5
, Ashish N. Rao , Miguel Castro , Thomas A. Cooper
1
1, 2, 3, 4 *
2
Departments of Integrative Molecular and Biomedical Sciences Program, Pathology and 3
4
Immunology, Molecular and Cellular Biology, Molecular Physiology and Biophysics, Baylor 5
College of Medicine, Houston, TX 77030, Bio-Synthesis, Inc., 612 East Main Street, Lewisville, TX 75057 *
corresponding author:
[email protected] ACS Paragon Plus Environment
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ABSTRACT Myotonic dystrophy type 1 (DM1) is a multisystemic disease caused by an expanded CTG repeat in the 3’ UTR of the dystrophia myotonica protein kinase (DMPK) gene. Short, DNA-based antisense oligonucleotides termed gapmers are a promising strategy to degrade toxic CUG expanded repeat (CUGexp) RNA. Nucleoside analogs are incorporated to increase gapmer affinity and stability, however some analogs also exhibit toxicity. In this study, we demonstrate that the NC
NC
2’,4’-BNA [NMe] (BNA ) modification is a promising nucleoside analog with high potency NC
similar to 2’,4’-LNA (LNA). BNA
gapmers targeting a non-repetitive region of the DMPK 3’ UTR
show allele-specific knockdown of CUGexp RNA and revert characteristic DM1 molecular defects NC
including mis-splicing and accumulation of RNA foci. Notably, the BNA
gapmers tested in this
study did not induce caspase activation, in contrast to a sequence matched LNA gapmer. This NC
study indicates BNA
gapmers warrant further study as a promising RNA targeting therapeutic.
INTRODUCTION Myotonic dystrophy is a multisystemic disease affecting approximately 1 in 8,000 individuals.(1) Myotonic dystrophy type I (DM1) is caused by a CTG repeat expansion within the 3’ UTR of the DMPK gene.(2,3) Expanded CUG repeat (CUGexp) RNA is retained in the nucleus and forms RNA foci that sequester the MBNL family of splicing factors and induces upregulation of CELF1 through PKC-mediated phosphorylation and altered microRNA regulation.(4-6) Altered MBNL and CELF1 activity in DM1 leads to defects in developmentally regulated alternative splicing.(1) Antisense oligonucleotides (ASOs) are a promising therapeutic approach for diseases caused by an RNA gain of function, including DM1. Addition of chemical modifications greatly stabilizes the affinity and stability of ASOs. These modifications include altered backbone chemistry, such as phosphorothioate (PS), and altered ribose chemistry, such as the 2’-Omethoxyethyl (MOE) and 2’-O,4’-C-methylene-bridged nucleic acid (LNA).(7) However, the addition of 2’ ribose modifications abolishes RNase H1-mediated target degradation.(8) Chimeric ASOs called gapmers contain 2’ ribose modifications at the 5’ and 3’ ends, leaving an internal 6– 10 nucleotide gap that maintains RNase H1 activity.(8-10) This is in contrast to mixmers, which contain modified analogs throughout the ASO and are unable to recruit RNase H1 for target cleavage (Figure S1A).(8) A recent clinical trial using a MOE gapmer (IONIS-DMPKRx) for the treatment of myotonic dystrophy demonstrated promise with the approach with current work focused on improving tissue delivery (Ionis Pharmaceuticals and Biogen press release, January 2017). Comparison of LNA and MOE gapmers indicates that LNA gapmers are 5–10 fold more potent, eliciting initial interest as a more potent alternative to MOE gapmers.(11,12) However, multiple studies have
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indicated that LNA gapmers induce RNase H1-dependent hepatotoxicity and apoptosis in both mice and cell models, reducing suitability for translational studies.(12-15) NC
NC
The 2’4’-BNA [NMe] (BNA ) modification was developed following similar principles as the LNA modification, with a bridged structure that greatly increases its affinity (Figure S1B).(16,17) NC
BNA
ASOs are more stable than LNA ASOs, and have been shown to be well tolerated in NC
mice.(16,18) However, BNA
gapmers have not been systematically tested in repeat expansion NC
models and it is unknown whether BNA NC
gapmers. We demonstrate that BNA
gapmers have similar toxicity concerns as LNA
gapmers have comparable potency to LNA gapmers,
display potentially lower propensity to induce caspase activity, and functionally rescue NC
characteristic DM1 defects, making BNA
gapmers a promising alternative chemistry for
therapeutic development.
RESULTS AND DISCUSSION NC
We first sought to compare the efficiency of BNA
and LNA gapmers at targeting DMPK
transcripts containing CUGexp. COSM6 cells were transfected with two plasmids: an rtTA expression plasmid and the pBitetDT700ctgGFP (Bi700CTG) plasmid, which contains a bidirectional tet-inducible promoter to express GFP and exons 11–15 of DMPK, including ~300 CUG repeats (Figure 1A). Twenty-four hours after plasmid transfection, cells were treated with NC
increasing concentrations of LNA or BNA
gapmers targeting either within the CUG repeat (CAG
gapmers) or in a non-repetitive region of DMPK (DMPK gapmers) (Figure 1; Table S1).(19) DMPK mRNA levels were quantified by RT-PCR relative to the GFP mRNA to standardize for NC
transfection efficiency. Compared to the CTG negative control gapmers, both LNA and BNA
CAG gapmers gave significant knockdown of CUGexp RNA at the lowest gapmer dose (0.3nM), and maximum knockdown to 65–80% of baseline at doses above 10nM (Figure 1C-D). We next NC
tested the efficiency of LNA and BNA
DMPK gapmers that target upstream of the expanded
repeat. While neither DMPK gapmer showed significant knockdown at the lowest dose, they both induced over 70% knockdown at 30nM. Interestingly, the DMPK gapmers displayed more potent knockdown than the CAG gapmers at the highest dose (100nM), with only 2–14% of the target NC
remaining (Figure 1C-D). The LNA DMPK gapmer was also more effective than the BNA
DMPK
gapmer at the low dosage levels. It is likely that the CAG gapmer is more effective than the DMPK gapmer at low concentrations because there are more binding sites per molecule. At higher concentrations, the residual amount of DMPK RNA that cannot be degraded by the CAG gapmer suggests the CUG repeat is partially protected, potentially by MBNL proteins or RNA NC
structure. Taken together, these results indicate that both LNA and BNA
gapmers are potent
and effective for knockdown of CUGexp RNA. NC
After establishing comparable potency between LNA and BNA NC
toxicity of BNA
gapmers, we compared the
and LNA gapmers. Non-DM1 TeloMyoD fibroblasts were treated with 30nM of
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NC
LNA or BNA
gapmers or mixmers and were assayed for membrane integrity, viability, and
caspase-3/7 activity 32 hours after transfection. We show a sequence-, chemistry- and RNase H1-dependent increased caspase response specifically caused by the LNA CAG gapmer and not NC
the BNA
CAG gapmer or the LNA CAG mixmer (Figure 2A, Figure S2A). Increased caspase
was not due to differences in cell number between samples because only the staurosporine treated cells showed a statistically significant decrease in viability (Figure 2B). Cytotoxicity was only elevated in cells treated with the positive control digitonin, indicating the ASOs tested do not display cytotoxic effects at 30nM (Figure S2B). Given that the LNA CAG mixmer did not elicit caspase activity, we hypothesized that LNA CAG gapmers induce caspase activity through on-target but non-desirable knockdown of nonNC
DMPK transcripts that contain CUG6+. However, we demonstrate that both LNA and BNA
CAG
gapmers induce RNase H1-mediated knockdown of all 11 tested CUG6+-containing mRNAs (Figure 2C, Figure S3). The question remains why LNA CAG gapmers induce caspase activity NC
but the sequence-matched BNA
CAG gapmers do not. Gapmer-mediated RNase H1 activity
includes off-target effects within intronic or exonic regions of long pre-mRNA transcripts.(14,20) Additionally, a variety of proteins bind ASOs and modulate their activity, and ASO chemistry can either promote or inhibit protein binding.(21,22) Therefore, differences in off-target effects or in the ASO-protein interactome could explain the differential caspase induction seen between the NC
LNA and BNA
CAG gapmers.
Previous work indicates that gapmers targeting within the repetitive region of DMPK preferentially degrade the mutant allele, and this region is an attractive target given the higher number of potential binding sites across the repeat tract.(23) However, given our results that nonDMPK transcripts containing short CUG repeat tracts were degraded by CAG gapmers, we NC
analyzed endogenous allele-specific RNA expression in DM1 cells after treatment with BNA gapmers. To distinguish between the expanded and non-expanded alleles we utilized a polymorphic site within DMPK and confirmed RNA transcripts from the expanded allele are NC
retained in the nucleus in these DM1 cells (Figure 3A-C).(24) Treatment with 30nM BNA
DMPK
gapmers induces preferential knockdown of the nuclear-retained CUGexp RNA without affecting the nuclear or cytoplasmic expression of the nonexpanded allele (Figure 3D-E). Unexpectedly, this preferential knockdown was not seen with the BNA
NC
CAG gapmer, which produced over
60% knockdown of total DMPK, but at the expense of targeting both the expanded and nonexpanded alleles (Figure 3E). In contrast, the BNA
NC
DMPK gapmer produced only 20%
knockdown of total DMPK, but this was largely accounted for by knockdown of the nuclearNC
retained, expanded allele. It is possible that the high potency of the BNA
gapmer saturated
knockdown of the expanded allele, leading to secondary degradation of the non-expanded DMPK mRNA. A recent study demonstrated that DMPK knockout mice do not have muscle or cardiac dysfunctions, making it possible that the CAG gapmer would still be viable for clinical
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translation.(25) However, the relative low specificity of this gapmer and higher toxicity seen for the LNA gapmer of this sequence indicate that targeting this repetitive region confers higher risk. NC
We next sought to determine whether BNA
gapmers could functionally rescue
characteristic defects in DM1 cells. First, we used fluorescent in situ hybridization (FISH) and NC
immunofluorescence (IF)-FISH to determine whether BNA
gapmers can reduce foci load and
release sequestered MBNL1. DM1 and non-DM1 TeloMyoD fibroblasts were treated with 30nM of NC
BNA
CAG or DMPK gapmers and differentiated for 6 days to induce the myogenic
program.(26,27) CUGexp RNA foci were visualized by RNA FISH (Figure S4A) and the number of foci per nucleus was quantified across three biological replicates (Figure 4A). Nearly all (97% ± 2.3%) of mock treated DM1 cells had nuclear RNA foci (Figure 4A, Figure S4C), while none of the 150 analyzed non-DM1 cells had nuclear foci. The total number of foci in 150 cells decreased NC
from 738 in DM1 mock treated cells, to 334 and 383 after treatment with BNA
CAG or DMPK
gapmers, respectively. This is reflected as a shift in the distribution of foci number per cell (Figure 4A). While over 30% of mock treated cells had more than 6 foci, only 5–7% of cells treated with NC
the BNA
CAG or DMPK gapmers had more than 6 foci. This effect was even more pronounced
in undifferentiated cells assayed 24 hours after gapmer treatment (Figure S4B-D). Partial foci knockdown, despite significant transcript knockdown by RT-PCR, may be a result of foci nucleation by a low absolute number of transcripts..(28) It is also possible that the MBNL-bound CUGexp RNA region is partially protected from exonuclease activity following RNase H1 cleavage. Given that the majority of cells still had at least one RNA focus after gapmer treatment, we were interested to determine the degree to which MBNL1 was released in cells that had decreased levels of RNA foci. We demonstrated that diffuse MBNL1 levels increased in the NC
nucleoplasm for cells treated with BNA NC
the BNA
CAG gapmers, however this result was not significant in
DMPK gapmers (Figure 4B-C and Figure S5). The increase in free MBNL1 is visible
even in cells that contain foci, indicating the presence of RNA foci is not necessarily a direct measure of MBNL1 availability. Our results in both differentiated and undifferentiated DM1 cells indicate that RNA foci are reduced and MBNL1 activity may be increased after treatment with NC
30nM of BNA
gapmers.
As RNA foci can be indicative of MBNL1 sequestration in DM1, we next analyzed whether NC
characteristic DM1 splicing abnormalities are rescued by BNA
gapmers. Differentiated DM1
TeloMyoD fibroblasts recapitulate splicing defects observed in DM1 skeletal muscle. Treatment of NC
these cells with 30nM of BNA
CAG or DMPK gapmers significantly reverted splicing of ALPK3,
MBNL1, and KIF13A towards the pattern in non-DM1 cells (Figure 4D). The splicing rescue for MBNL1 and KIF13A was robust while rescue was more moderate for the less severely affected event ALPK3. The level of splicing rescue for these events is notable, especially given the residual number of about 1–3 foci per cell after gapmer treatment. This suggests that decreased
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foci load can be sufficient to revert splicing without complete degradation of all RNA foci and NC
demonstrates that BNA
gapmers potently revert splicing defects in DM1 cells. NC
In conclusion, we have shown that BNA
gapmers are a promising therapeutic option to NC
target toxic RNA in myotonic dystrophy. The allele-specific knockdown achieved with the BNA
DMPK, but not CAG, gapmers indicates targeting a non-repetitive region improves preferential knockdown of the expanded allele. Determining the mechanism responsible for differences in NC
caspase induction between LNA and BNA
CAG gapmers is a key area of interest and will aid in
overcoming toxicity concerns for future gapmer-based therapies.
METHODS NC
Antisense oligonucleotides. LNA and BNA
ASOs were purchased from Exiqon and Bio-
Synthesis, respectively.
Cell models and assays SB TeloMyoD (control, non-DM1) and KB TeloMyoD (DM1, 400 CTG repeats) immortalized human fibroblast cell lines express telomerase and contain a tetracycline-inducible MyoD to promote the myogenic program in response to growth for 6 days in low serum media (1% FBS) supplemented with 1 µg/ml doxycycline.(26,27) Toxicity analyses were conducted using the ApoTox-Glo Triplex Assay (Promega). Additional assay details and RT-PCR primers are listed in Supplementary Data and Table S2.
Microscopy TeloMyoD fibroblasts were electroporated with 30nM of gapmers, differentiated for 6 days and visualized by RNA FISH using the (CAG)5 TYE 563 LNA probe (CAGCAGCAGCAGCAG) or by IF/FISH using MBNL1 (Santa Cruz, sc-47740). For further details see Supplementary Data.
Statistical analysis Data is expressed as mean ± standard deviation. All data shown is the summary of three or more biological replicates and statistical analyses were completed in Prism 7. For datasets where three or more groups were analyzed simultaneously, one-way ANOVA was used with ungrouped data and two-way ANOVA was used with grouped data and were corrected for multiple comparisons. Statistical values used: *P
