Ravi Kumar Sindhu scite author profile

Ravi Kumar Sindhu

4Publications

50Citation Statements Received

122Citation Statements Given

How they've been cited

How they cite others

121

Affiliations

National Institute on Alcohol Abuse and Alcoholism, Walter Reed Army Institute of Research, Henry M. Jackson Foundation

Publications

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Early rearing history influences oxytocin receptor epigenetic regulation in rhesus macaques

Baker

Lindell

Driscoll

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

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SignificanceEpigenetically programmed stress adaptation may be a conduit for informing offspring of environmental challenge. We employed ChIP-sequencing to examine effects of early environment on epigenetic regulation using hippocampal samples from macaques exposed to disruption in maternal care. We found decreased H3K4me3 binding at genes critical to behavioral stress response, the most robust being the oxytocin receptor gene (OXTR), for which we observed a corresponding decrease in RNA expression. Post hoc analysis showed that a gain-of-function OXTR SNP rescued behavioral differences in early stress-exposed subjects. Our data suggest that epigenetic down-modulation of OXTR in brain could contribute to behavioral differences observed in early stress-exposed subjects and that functional genetic variation plays a role. These could have translational implications for human psychiatric disease and personality disorders.

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High‐throughput next‐generation sequencing to genotype six classical HLA loci from 96 donors in a single MiSeq run

Ehrenberg

Geretz

Sindhu

et al. 2017

HLA

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Next generation sequencing (NGS) methods have been established as an efficient approach for HLA typing because unlike traditional Sanger sequencing, they provide unambiguous results at a reasonable cost. We previously developed a multi-locus index method to genotype four HLA loci (A, B, C, and DRB1) on the Illumina MiSeq platform. We have now expanded this method to include two additional loci, HLA-DPB1 and DQB1. Contiguous full-length amplicons from 5'UTR through 3'UTR regions were generated using one long-range PCR reaction per locus for each of the six loci from 96 individuals of different ethnicities. The six amplicons from each donor were pooled, enzymatically fragmented and given a donor-specific index. This approach enabled sequencing of 576 loci from 96 individuals in a single MiSeq run. Donor-specific sequence reads were demultiplexed, and allele calls were generated from FASTQ files using commercially available software. Comparison to HLA genotypes generated from Sanger sequence-based typing (SBT) identified no discordances among any of the alleles analyzed in this study. Importantly, this method was able to resolve 22 DPB1 and 20 DQB1 alleles that were ambiguous with the SBT method. Furthermore, a novel allele in each of these two loci was identified, with the DQB1*05:01:24 allele having a frequency of greater than five percent. This method was subsequently validated against a blinded panel of 22 samples from the 17th International HLA and Immunogenetics Workshop. The flexibility of the method is further highlighted by successful genotyping of eight loci comprising all classical HLA loci for a subset of the samples. We now present a high-throughput, high-resolution, scalable NGS HLA typing method to accurately and efficiently genotype all classical HLA class I and II loci.

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Growth of Streptococcus pneumoniae on Macconkey Agar: Possibility of Impossible?

Ranjan

Bakthavathsalam

Raghavan

et al. 2014

JCDR

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P037 Genotyping of six classical HLA loci using next generation sequencing

et al. 2016

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