Your search keyword '"Patwardhan RP"' showing total 11 results

1. Systematic Dissection of Coding Exons at Single Nucleotide Resolution Supports an Additional Role in Cell-Specific Transcriptional Regulation

Author

Ahituv, Nadav, Birnbaum, RY, Patwardhan, RP, Kim, MJ, Findlay, GM, Martin, B, Zhao, J, Bell, RJA, Smith, RP, Ku, AA, and Shendure, J

Abstract

© 2014 Birnbaum et al.In addition to their protein coding function, exons can also serve as transcriptional enhancers. Mutations in these exonic-enhancers (eExons) could alter both protein function and transcription. However, the functional consequence of

Published

2014

2. The Rhododendron Genome and Chromosomal Organization Provide Insight into Shared Whole-Genome Duplications across the Heath Family (Ericaceae).

Author

Soza VL, Lindsley D, Waalkes A, Ramage E, Patwardhan RP, Burton JN, Adey A, Kumar A, Qiu R, Shendure J, and Hall B

Subjects

Base Sequence, Chromatin genetics, Chromosome Mapping, Genetic Linkage, Genomic Library, Molecular Sequence Annotation, Transposases genetics, Chromosomes, Plant genetics, Ericaceae genetics, Genome, Plant genetics, Rhododendron genetics, Synteny

Abstract

The genus Rhododendron (Ericaceae), which includes horticulturally important plants such as azaleas, is a highly diverse and widely distributed genus of >1,000 species. Here, we report the chromosome-scale de novo assembly and genome annotation of Rhododendron williamsianum as a basis for continued study of this large genus. We created multiple short fragment genomic libraries, which were assembled using ALLPATHS-LG. This was followed by contiguity preserving transposase sequencing (CPT-seq) and fragScaff scaffolding of a large fragment library, which improved the assembly by decreasing the number of scaffolds and increasing scaffold length. Chromosome-scale scaffolding was performed by proximity-guided assembly (LACHESIS) using chromatin conformation capture (Hi-C) data. Chromosome-scale scaffolding was further refined and linkage groups defined by restriction-site associated DNA (RAD) sequencing of the parents and progeny of a genetic cross. The resulting linkage map confirmed the LACHESIS clustering and ordering of scaffolds onto chromosomes and rectified large-scale inversions. Assessments of the R. williamsianum genome assembly and gene annotation estimate them to be 89% and 79% complete, respectively. Predicted coding sequences from genome annotation were used in syntenic analyses and for generating age distributions of synonymous substitutions/site between paralgous gene pairs, which identified whole-genome duplications (WGDs) in R. williamsianum. We then analyzed other publicly available Ericaceae genomes for shared WGDs. Based on our spatial and temporal analyses of paralogous gene pairs, we find evidence for two shared, ancient WGDs in Rhododendron and Vaccinium (cranberry/blueberry) members that predate the Ericaceae family and, in one case, the Ericales order., (© The Author(s) 2019. Published by Oxford University Press on behalf of the Society for Molecular Biology and Evolution.)

Published

2019

3. Learning the sequence determinants of alternative splicing from millions of random sequences.

Author

Rosenberg AB, Patwardhan RP, Shendure J, and Seelig G

Subjects

Base Sequence, Humans, Molecular Sequence Data, Nucleotide Motifs, RNA Splice Sites, Alternative Splicing, Genome, Human, Models, Genetic, Polymorphism, Single Nucleotide

Abstract

Most human transcripts are alternatively spliced, and many disease-causing mutations affect RNA splicing. Toward better modeling the sequence determinants of alternative splicing, we measured the splicing patterns of over two million (M) synthetic mini-genes, which include degenerate subsequences totaling over 100 M bases of variation. The massive size of these training data allowed us to improve upon current models of splicing, as well as to gain new mechanistic insights. Our results show that the vast majority of hexamer sequence motifs measurably influence splice site selection when positioned within alternative exons, with multiple motifs acting additively rather than cooperatively. Intriguingly, motifs that enhance (suppress) exon inclusion in alternative 5' splicing also enhance (suppress) exon inclusion in alternative 3' or cassette exon splicing, suggesting a universal mechanism for alternative exon recognition. Finally, our empirically trained models are highly predictive of the effects of naturally occurring variants on alternative splicing in vivo., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

4. Systematic dissection of coding exons at single nucleotide resolution supports an additional role in cell-specific transcriptional regulation.

Author

Birnbaum RY, Patwardhan RP, Kim MJ, Findlay GM, Martin B, Zhao J, Bell RJ, Smith RP, Ku AA, Shendure J, and Ahituv N

Subjects

Animals, Binding Sites, Gene Expression Regulation, HeLa Cells, Humans, Liver metabolism, Mice, Mutation, Missense, Polymorphism, Single Nucleotide, RNA Splicing genetics, Transcription Factors biosynthesis, Adaptor Proteins, Signal Transducing genetics, Enhancer Elements, Genetic, Exons genetics, Membrane Transport Proteins genetics, PPAR gamma genetics, Receptors, LDL genetics

Abstract

In addition to their protein coding function, exons can also serve as transcriptional enhancers. Mutations in these exonic-enhancers (eExons) could alter both protein function and transcription. However, the functional consequence of eExon mutations is not well known. Here, using massively parallel reporter assays, we dissect the enhancer activity of three liver eExons (SORL1 exon 17, TRAF3IP2 exon 2, PPARG exon 6) at single nucleotide resolution in the mouse liver. We find that both synonymous and non-synonymous mutations have similar effects on enhancer activity and many of the deleterious mutation clusters overlap known liver-associated transcription factor binding sites. Carrying a similar massively parallel reporter assay in HeLa cells with these three eExons found differences in their mutation profiles compared to the liver, suggesting that enhancers could have distinct operating profiles in different tissues. Our results demonstrate that eExon mutations could lead to multiple phenotypes by disrupting both the protein sequence and enhancer activity and that enhancers can have distinct mutation profiles in different cell types.

Published

2014

5. Chromosome-scale scaffolding of de novo genome assemblies based on chromatin interactions.

Author

Burton JN, Adey A, Patwardhan RP, Qiu R, Kitzman JO, and Shendure J

Subjects

Animals, Base Sequence, Drosophila, Humans, Mice, Molecular Sequence Data, Algorithms, Chromatin genetics, Chromosome Mapping methods, Contig Mapping methods, Sequence Analysis, DNA methods

Abstract

Genomes assembled de novo from short reads are highly fragmented relative to the finished chromosomes of Homo sapiens and key model organisms generated by the Human Genome Project. To address this problem, we need scalable, cost-effective methods to obtain assemblies with chromosome-scale contiguity. Here we show that genome-wide chromatin interaction data sets, such as those generated by Hi-C, are a rich source of long-range information for assigning, ordering and orienting genomic sequences to chromosomes, including across centromeres. To exploit this finding, we developed an algorithm that uses Hi-C data for ultra-long-range scaffolding of de novo genome assemblies. We demonstrate the approach by combining shotgun fragment and short jump mate-pair sequences with Hi-C data to generate chromosome-scale de novo assemblies of the human, mouse and Drosophila genomes, achieving--for the human genome--98% accuracy in assigning scaffolds to chromosome groups and 99% accuracy in ordering and orienting scaffolds within chromosome groups. Hi-C data can also be used to validate chromosomal translocations in cancer genomes.

Published

2013

6. Massively parallel decoding of mammalian regulatory sequences supports a flexible organizational model.

Author

Smith RP, Taher L, Patwardhan RP, Kim MJ, Inoue F, Shendure J, Ovcharenko I, and Ahituv N

Subjects

Animals, Binding Sites, Cell Line, Cluster Analysis, Enhancer Elements, Genetic, Gene Amplification, Gene Dosage, Gene Expression, Genes, Reporter, Humans, Liver metabolism, Male, Mice, Nucleotide Motifs, Organ Specificity genetics, Protein Binding, Gene Expression Regulation, Models, Biological, Regulatory Sequences, Nucleic Acid, Transcription Factors metabolism

Abstract

Despite continual progress in the cataloging of vertebrate regulatory elements, little is known about their organization and regulatory architecture. Here we describe a massively parallel experiment to systematically test the impact of copy number, spacing, combination and order of transcription factor binding sites on gene expression. A complex library of ∼5,000 synthetic regulatory elements containing patterns from 12 liver-specific transcription factor binding sites was assayed in mice and in HepG2 cells. We find that certain transcription factors act as direct drivers of gene expression in homotypic clusters of binding sites, independent of spacing between sites, whereas others function only synergistically. Heterotypic enhancers are stronger than their homotypic analogs and favor specific transcription factor binding site combinations, mimicking putative native enhancers. Exhaustive testing of binding site permutations suggests that there is flexibility in binding site order. Our findings provide quantitative support for a flexible model of regulatory element activity and suggest a framework for the design of synthetic tissue-specific enhancers.

Published

2013

7. Massively parallel functional dissection of mammalian enhancers in vivo.

Author

Patwardhan RP, Hiatt JB, Witten DM, Kim MJ, Smith RP, May D, Lee C, Andrie JM, Lee SI, Cooper GM, Ahituv N, Pennacchio LA, and Shendure J

Subjects

Animals, Binding Sites, Evolution, Molecular, Genes, Reporter, Haplotypes, Humans, Linear Models, Liver metabolism, Mice, Mutagenesis, Mutation, Transcription Factors metabolism, Transcription, Genetic, Enhancer Elements, Genetic, Transcription Factors genetics

Abstract

The functional consequences of genetic variation in mammalian regulatory elements are poorly understood. We report the in vivo dissection of three mammalian enhancers at single-nucleotide resolution through a massively parallel reporter assay. For each enhancer, we synthesized a library of >100,000 mutant haplotypes with 2-3% divergence from the wild-type sequence. Each haplotype was linked to a unique sequence tag embedded within a transcriptional cassette. We introduced each enhancer library into mouse liver and measured the relative activities of individual haplotypes en masse by sequencing the transcribed tags. Linear regression analysis yielded highly reproducible estimates of the effect of every possible single-nucleotide change on enhancer activity. The functional consequence of most mutations was modest, with ∼22% affecting activity by >1.2-fold and ∼3% by >2-fold. Several, but not all, positions with higher effects showed evidence for purifying selection, or co-localized with known liver-associated transcription factor binding sites, demonstrating the value of empirical high-resolution functional analysis.

Published

2012

8. The ecoresponsive genome of Daphnia pulex.

Author

Colbourne JK, Pfrender ME, Gilbert D, Thomas WK, Tucker A, Oakley TH, Tokishita S, Aerts A, Arnold GJ, Basu MK, Bauer DJ, Cáceres CE, Carmel L, Casola C, Choi JH, Detter JC, Dong Q, Dusheyko S, Eads BD, Fröhlich T, Geiler-Samerotte KA, Gerlach D, Hatcher P, Jogdeo S, Krijgsveld J, Kriventseva EV, Kültz D, Laforsch C, Lindquist E, Lopez J, Manak JR, Muller J, Pangilinan J, Patwardhan RP, Pitluck S, Pritham EJ, Rechtsteiner A, Rho M, Rogozin IB, Sakarya O, Salamov A, Schaack S, Shapiro H, Shiga Y, Skalitzky C, Smith Z, Souvorov A, Sung W, Tang Z, Tsuchiya D, Tu H, Vos H, Wang M, Wolf YI, Yamagata H, Yamada T, Ye Y, Shaw JR, Andrews J, Crease TJ, Tang H, Lucas SM, Robertson HM, Bork P, Koonin EV, Zdobnov EM, Grigoriev IV, Lynch M, and Boore JL

Subjects

Adaptation, Physiological, Amino Acid Sequence, Animals, Base Sequence, Chromosome Mapping, Daphnia physiology, Environment, Evolution, Molecular, Gene Conversion, Gene Duplication, Gene Expression, Gene Expression Profiling, Gene Expression Regulation, Genes, Genes, Duplicate, Metabolic Networks and Pathways genetics, Molecular Sequence Annotation, Molecular Sequence Data, Multigene Family, Phylogeny, Sequence Analysis, DNA, Daphnia genetics, Ecosystem, Genome

Abstract

We describe the draft genome of the microcrustacean Daphnia pulex, which is only 200 megabases and contains at least 30,907 genes. The high gene count is a consequence of an elevated rate of gene duplication resulting in tandem gene clusters. More than a third of Daphnia's genes have no detectable homologs in any other available proteome, and the most amplified gene families are specific to the Daphnia lineage. The coexpansion of gene families interacting within metabolic pathways suggests that the maintenance of duplicated genes is not random, and the analysis of gene expression under different environmental conditions reveals that numerous paralogs acquire divergent expression patterns soon after duplication. Daphnia-specific genes, including many additional loci within sequenced regions that are otherwise devoid of annotations, are the most responsive genes to ecological challenges.

Published

2011

9. Haplotype-resolved genome sequencing of a Gujarati Indian individual.

Author

Kitzman JO, Mackenzie AP, Adey A, Hiatt JB, Patwardhan RP, Sudmant PH, Ng SB, Alkan C, Qiu R, Eichler EE, and Shendure J

Subjects

Base Sequence, Cell Line, Heterozygote, Humans, Models, Molecular, Polymorphism, Single Nucleotide genetics, Asian People genetics, Genome, Human genetics, Haplotypes genetics, High-Throughput Nucleotide Sequencing methods, Sequence Analysis, DNA methods

Abstract

Haplotype information is essential to the complete description and interpretation of genomes, genetic diversity and genetic ancestry. Although individual human genome sequencing is increasingly routine, nearly all such genomes are unresolved with respect to haplotype. Here we combine the throughput of massively parallel sequencing with the contiguity information provided by large-insert cloning to experimentally determine the haplotype-resolved genome of a South Asian individual. A single fosmid library was split into a modest number of pools, each providing ∼3% physical coverage of the diploid genome. Sequencing of each pool yielded reads overwhelmingly derived from only one homologous chromosome at any given location. These data were combined with whole-genome shotgun sequence to directly phase 94% of ascertained heterozygous single nucleotide polymorphisms (SNPs) into long haplotype blocks (N50 of 386 kilobases (kbp)). This method also facilitates the analysis of structural variation, for example, to anchor novel insertions to specific locations and haplotypes.

Published

2011

10. Parallel, tag-directed assembly of locally derived short sequence reads.

Author

Hiatt JB, Patwardhan RP, Turner EH, Lee C, and Shendure J

Subjects

Base Sequence, Expressed Sequence Tags, Molecular Sequence Data, Chromosome Mapping methods, Sequence Analysis, DNA methods

Abstract

We demonstrate subassembly, an in vitro library construction method that extends the utility of short-read sequencing platforms to applications requiring long, accurate reads. A long DNA fragment library is converted to a population of nested sublibraries, and a tag sequence directs grouping of short reads derived from the same long fragment, enabling localized assembly of long fragment sequences. Subassembly may facilitate accurate de novo genome assembly and metagenome sequencing.

Published

2010

11. High-resolution analysis of DNA regulatory elements by synthetic saturation mutagenesis.

Author

Patwardhan RP, Lee C, Litvin O, Young DL, Pe'er D, and Shendure J

Subjects

Base Sequence, Molecular Sequence Data, Algorithms, DNA chemistry, DNA genetics, Mutagenesis, Site-Directed methods, Regulatory Elements, Transcriptional genetics, Sequence Analysis, DNA methods

Abstract

We present a method that harnesses massively parallel DNA synthesis and sequencing for the high-throughput functional analysis of regulatory sequences at single-nucleotide resolution. As a proof of concept, we quantitatively assayed the effects of all possible single-nucleotide mutations for three bacteriophage promoters and three mammalian core promoters in a single experiment per promoter. The method may also serve as a rapid screening tool for regulatory element engineering in synthetic biology.

Published

2009