Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)

Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)

<p>Abstract</p> <p>Background</p> <p>Four genes designated as PTPRK (PTPκ), PTPRL/U (PCP-2), PTPRM (PTPμ) and PTPRT (PTPρ) code for a subfamily (type R2B) of receptor protein tyrosine phosphatases (RPTPs) uniquely characterized by the presence of an N-terminal MAM domai...

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Main Authors: Frostholm Adrienne, Davuluri Ramana V, Popesco Magdalena C, Besco Julie, Rotter Andrej
Format: Article
Language:English
Published: BMC 2004-02-01
Series:BMC Genomics
Subjects:
central nervous system
dephosphorylation
alternative splicing
adhesion molecules
Online Access:http://www.biomedcentral.com/1471-2164/5/14
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spelling doaj-b3694d3f03f24d3bb1b778132088050c2020-11-24T22:57:08ZengBMCBMC Genomics1471-21642004-02-01511410.1186/1471-2164-5-14Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)Frostholm AdrienneDavuluri Ramana VPopesco Magdalena CBesco JulieRotter Andrej<p>Abstract</p> <p>Background</p> <p>Four genes designated as PTPRK (PTPκ), PTPRL/U (PCP-2), PTPRM (PTPμ) and PTPRT (PTPρ) code for a subfamily (type R2B) of receptor protein tyrosine phosphatases (RPTPs) uniquely characterized by the presence of an N-terminal MAM domain. These transmembrane molecules have been implicated in homophilic cell adhesion. In the human, the PTPRK gene is located on chromosome 6, PTPRL/U on 1, PTPRM on 18 and PTPRT on 20. In the mouse, the four genes <it>ptprk, ptprl, ptprm </it>and <it>ptprt </it>are located in syntenic regions of chromosomes 10, 4, 17 and 2, respectively.</p> <p>Results</p> <p>The genomic organization of murine R2B RPTP genes is described. The four genes varied greatly in size ranging from ~64 kb to ~1 Mb, primarily due to proportional differences in intron lengths. Although there were also minor variations in exon length, the number of exons and the phases of exon/intron junctions were highly conserved. In situ hybridization with digoxigenin-labeled cRNA probes was used to localize each of the four R2B transcripts to specific cell types within the murine central nervous system. Phylogenetic analysis of complete sequences indicated that PTPρ and PTPμ were most closely related, followed by PTPκ. The most distant family member was PCP-2. Alignment of RPTP polypeptide sequences predicted putative alternatively spliced exons. PCR experiments revealed that five of these exons were alternatively spliced, and that each of the four phosphatases incorporated them differently. The greatest variability in genomic organization and the majority of alternatively spliced exons were observed in the juxtamembrane domain, a region critical for the regulation of signal transduction.</p> <p>Conclusions</p> <p>Comparison of the four R2B RPTP genes revealed virtually identical principles of genomic organization, despite great disparities in gene size due to variations in intron length. Although subtle differences in exon length were also observed, it is likely that functional differences among these genes arise from the specific combinations of exons generated by alternative splicing.</p> http://www.biomedcentral.com/1471-2164/5/14central nervous systemdephosphorylationalternative splicingadhesion molecules
collection DOAJ
language English
format Article
sources DOAJ
author Frostholm Adrienne
Davuluri Ramana V
Popesco Magdalena C
Besco Julie
Rotter Andrej
spellingShingle Frostholm Adrienne
Davuluri Ramana V
Popesco Magdalena C
Besco Julie
Rotter Andrej
Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
BMC Genomics
central nervous system
dephosphorylation
alternative splicing
adhesion molecules
author_facet Frostholm Adrienne
Davuluri Ramana V
Popesco Magdalena C
Besco Julie
Rotter Andrej
author_sort Frostholm Adrienne
title Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
title_short Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
title_full Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
title_fullStr Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
title_full_unstemmed Genomic structure and alternative splicing of murine R2B receptor protein tyrosine phosphatases (PTPκ, μ, ρ and PCP-2)
title_sort genomic structure and alternative splicing of murine r2b receptor protein tyrosine phosphatases (ptpκ, μ, ρ and pcp-2)
publisher BMC
series BMC Genomics
issn 1471-2164
publishDate 2004-02-01
description <p>Abstract</p> <p>Background</p> <p>Four genes designated as PTPRK (PTPκ), PTPRL/U (PCP-2), PTPRM (PTPμ) and PTPRT (PTPρ) code for a subfamily (type R2B) of receptor protein tyrosine phosphatases (RPTPs) uniquely characterized by the presence of an N-terminal MAM domain. These transmembrane molecules have been implicated in homophilic cell adhesion. In the human, the PTPRK gene is located on chromosome 6, PTPRL/U on 1, PTPRM on 18 and PTPRT on 20. In the mouse, the four genes <it>ptprk, ptprl, ptprm </it>and <it>ptprt </it>are located in syntenic regions of chromosomes 10, 4, 17 and 2, respectively.</p> <p>Results</p> <p>The genomic organization of murine R2B RPTP genes is described. The four genes varied greatly in size ranging from ~64 kb to ~1 Mb, primarily due to proportional differences in intron lengths. Although there were also minor variations in exon length, the number of exons and the phases of exon/intron junctions were highly conserved. In situ hybridization with digoxigenin-labeled cRNA probes was used to localize each of the four R2B transcripts to specific cell types within the murine central nervous system. Phylogenetic analysis of complete sequences indicated that PTPρ and PTPμ were most closely related, followed by PTPκ. The most distant family member was PCP-2. Alignment of RPTP polypeptide sequences predicted putative alternatively spliced exons. PCR experiments revealed that five of these exons were alternatively spliced, and that each of the four phosphatases incorporated them differently. The greatest variability in genomic organization and the majority of alternatively spliced exons were observed in the juxtamembrane domain, a region critical for the regulation of signal transduction.</p> <p>Conclusions</p> <p>Comparison of the four R2B RPTP genes revealed virtually identical principles of genomic organization, despite great disparities in gene size due to variations in intron length. Although subtle differences in exon length were also observed, it is likely that functional differences among these genes arise from the specific combinations of exons generated by alternative splicing.</p>
topic central nervous system
dephosphorylation
alternative splicing
adhesion molecules
url http://www.biomedcentral.com/1471-2164/5/14
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