Literature DB >> 26216192

Functional Networks of Highest-Connected Splice Isoforms: From The Chromosome 17 Human Proteome Project.

Hong-Dong Li1, Rajasree Menon1, Brandon Govindarajoo1, Bharat Panwar1, Yang Zhang1, Gilbert S Omenn1, Yuanfang Guan1.   

Abstract

Alternative splicing allows a single gene to produce multiple transcript-level splice isoforms from which the translated proteins may show differences in their expression and function. Identifying the major functional or canonical isoform is important for understanding gene and protein functions. Identification and characterization of splice isoforms is a stated goal of the HUPO Human Proteome Project and of neXtProt. Multiple efforts have catalogued splice isoforms as "dominant", "principal", or "major" isoforms based on expression or evolutionary traits. In contrast, we recently proposed highest connected isoforms (HCIs) as a new class of canonical isoforms that have the strongest interactions in a functional network and revealed their significantly higher (differential) transcript-level expression compared to nonhighest connected isoforms (NCIs) regardless of tissues/cell lines in the mouse. HCIs and their expression behavior in the human remain unexplored. Here we identified HCIs for 6157 multi-isoform genes using a human isoform network that we constructed by integrating a large compendium of heterogeneous genomic data. We present examples for pairs of transcript isoforms of ABCC3, RBM34, ERBB2, and ANXA7. We found that functional networks of isoforms of the same gene can show large differences. Interestingly, differential expression between HCIs and NCIs was also observed in the human on an independent set of 940 RNA-seq samples across multiple tissues, including heart, kidney, and liver. Using proteomic data from normal human retina and placenta, we showed that HCIs are a promising indicator of expressed protein isoforms exemplified by NUDFB6 and M6PR. Furthermore, we found that a significant percentage (20%, p = 0.0003) of human and mouse HCIs are homologues, suggesting their conservation between species. Our identified HCIs expand the repertoire of canonical isoforms and are expected to facilitate studying main protein products, understanding gene regulation, and possibly evolution. The network is available through our web server as a rich resource for investigating isoform functional relationships (http://guanlab.ccmb.med.umich.edu/hisonet). All MS/MS data were available at ProteomeXchange Web site (http://www.proteomexchange.org) through their identifiers (retina: PXD001242, placenta: PXD000754).

Entities:  

Keywords:  alternative splicing; canonical isoforms; highest connected isoforms; isoform networks

Mesh:

Substances:

Year:  2015        PMID: 26216192      PMCID: PMC4993635          DOI: 10.1021/acs.jproteome.5b00494

Source DB:  PubMed          Journal:  J Proteome Res        ISSN: 1535-3893            Impact factor:   4.466


  46 in total

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4.  Odd-skipped related 2 splicing variants show opposite transcriptional activity.

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6.  Tissue-specific functional networks for prioritizing phenotype and disease genes.

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  16 in total

1.  A proteogenomic approach to understand splice isoform functions through sequence and expression-based computational modeling.

Authors:  Hong-Dong Li; Gilbert S Omenn; Yuanfang Guan
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2.  Annotation of Alternatively Spliced Proteins and Transcripts with Protein-Folding Algorithms and Isoform-Level Functional Networks.

Authors:  Hongdong Li; Yang Zhang; Yuanfang Guan; Rajasree Menon; Gilbert S Omenn
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Review 5.  Alternative Splicing May Not Be the Key to Proteome Complexity.

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8.  Assessing the functional relevance of splice isoforms.

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Journal:  Alzheimers Dement       Date:  2021-01-21       Impact factor: 21.566

10.  A Network of Splice Isoforms for the Mouse.

Authors:  Hong-Dong Li; Rajasree Menon; Ridvan Eksi; Aysam Guerler; Yang Zhang; Gilbert S Omenn; Yuanfang Guan
Journal:  Sci Rep       Date:  2016-04-15       Impact factor: 4.379

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