نتایج جستجو برای: splice site

تعداد نتایج: 363045  

Journal: :The EMBO journal 1999
M Blanchette B Chabot

The RNA-binding protein hnRNP A1 is a splicing regulator produced by exclusion of alternative exon 7B from the A1 pre-mRNA. Each intron flanking exon 7B contains a high-affinity A1-binding site. The A1-binding elements promote exon skipping in vivo, activate distal 5' splice site selection in vitro and improve the responsiveness of pre-mRNAs to increases in the concentration of A1. Whereas the ...

Journal: :Journal of medical genetics 2005
T Rossenbacker E Schollen C Kuipéri T J L de Ravel K Devriendt G Matthijs D Collen H Heidbüchel P Carmeliet

BACKGROUND Mutations in the cardiac sodium channel, SCN5A, have been associated with one type of long-QT syndrome, with isolated cardiac conduction defects and Brugada syndrome. The sodium channelopathies exhibit marked variation in clinical phenotypes. The mechanisms underlying the phenotypical diversity, however, remain unknown. Exonic SCN5A mutations can be detected in 20% of Brugada syndrom...

Journal: :Nucleic acids research 1994
S Stamm M Q Zhang T G Marr D M Helfman

Alternative splicing is an important regulatory mechanism to create protein diversity. In order to elucidate possible regulatory elements common to neuron specific exons, we created and statistically analysed a database of exons that are alternatively spliced in neurons. The splice site comparison of alternatively and constitutively spliced exons reveals that some, but not all alternatively spl...

Journal: :Nucleic acids research 2004
Rachel Flomen Joanne Knight Pak Sham Robert Kerwin Andrew Makoff

Adenosine to inosine editing of mRNA from the human 5-HT2C receptor gene (HTR2C) occurs at five exonic positions (A-E) in a stable stem-loop that includes the normal 5' splice site of intron 5 and is flanked by two alternative splice sites. Using in vitro editing, we identified a novel editing site (F) located in the intronic part of the stem-loop and demonstrated editing at this site in human ...

2010
Chongfei Jin Jin Jiang Wei Wang Ke Yao

PURPOSE To investigate the consequence of a major intrinsic protein MIP splice-site mutation (c.607-1G>A) in a four-generation Chinese pedigree afflicted with autosomal dominant congenital cataracts (ADCC). METHODS Both a mutated minigene with c.607-1G>A, and a wild-type minigene were constructed using the pTARGET mammalian expression vector. They were transiently transfected into HeLa cells ...

Journal: :Molecular and cellular biology 1997
C F Kennedy S M Berget

The minimum size for splicing of a vertebrate intron is approximately 70 nucleotides. In Drosophila melanogaster, more than half of the introns are significantly below this minimum yet function well. Such short introns often lack the pyrimidine tract located between the branch point and 3' splice site common to metazoan introns. To investigate if small introns contain special sequences that fac...

Journal: :Genome informatics. International Conference on Genome Informatics 2003
Loi Sy Ho Jagath C Rajapakse

The performance of the ab inito gene prediction approaches mostly depends on the effectiveness of detecting the splice sites. This paper addresses the problem of splice site detection using higher-order Markov models. The tenet of our approach is to brace the higher-order dependencies of a Markov model by a neural network that receives the inputs from low-order Markov chains. The method is able...

Journal: :Molecular and cellular biology 2005
Haixin Lei Igor Vorechovsky

Auxiliary splicing signals in introns play an important role in splice site selection, but these elements are poorly understood. We show that a subset of serine/arginine (SR)-rich proteins activate a cryptic 3' splice site in a sense Alu repeat located in intron 4 of the human LST1 gene. Utilization of this cryptic splice site is controlled by juxtaposed Alu-derived splicing silencers and enhan...

2007
Kenjyo Miyauchi Tomoya Ohara Tsutomu Suzuki

Results A method for predicting trans-splicing sites must be able to identify more than one likely splice site in a given trans-splicing region if the conditions warrant such a prediction. Otherwise, the predictive ability of the method would be limited to identifying one of several possible splice sites. Therefore, we wished to assess our method’s predictive ability on a set of known trans-spl...

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