Literature DB >> 8290351

Stimulation of gene expression by introns: conversion of an inhibitory intron to a stimulatory intron by alteration of the splice donor sequence.

M Korb1, Y Ke, L F Johnson.   

Abstract

Efficient expression of many mammalian genes depends on the presence of at least one intron. We previously showed that addition of almost any of the introns from the mouse thymidylate synthase (TS) gene to an intronless TS minigene led to a large increase in expression. However, addition of intron 4 led to a reduction in minigene expression. The goal of the present study was to determine why TS intron 4 was unable to stimulate expression. Insertion of intron 4 into an intron-dependent derivative of the ribosomal protein L32 gene did not lead to a significant increase in expression, suggesting that its inability to stimulate expression was due to sequences within the intron. Deleting most of the interior of intron 4, improving the putative branch point, removing purines from the pyrimidine stretch at the 3' end of the intron, or removing possible alternative splice acceptor or donor sites within the intron each had little effect on the level of expression. However, when the splice donor sequence of intron 4 was modified so that it was perfectly complementary to U1 snRNA, the modified intron 4 stimulated expression approximately 6-fold. When the splice donor site of TS intron 1 (a stimulatory intron) was changed to that of TS intron 4, the modified intron 1 was spliced very inefficiently and lost the ability to stimulate mRNA production. Our observations support the idea that introns can stimulate gene expression by a process that depends directly on the splicing reaction.

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Year:  1993        PMID: 8290351      PMCID: PMC310472          DOI: 10.1093/nar/21.25.5901

Source DB:  PubMed          Journal:  Nucleic Acids Res        ISSN: 0305-1048            Impact factor:   16.971


  63 in total

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Authors:  S L McKnight
Journal:  Nucleic Acids Res       Date:  1980-12-20       Impact factor: 16.971

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5.  A lymphocyte-specific cellular enhancer is located downstream of the joining region in immunoglobulin heavy chain genes.

Authors:  J Banerji; L Olson; W Schaffner
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Review 6.  The organization and expression of histone gene families.

Authors:  C C Hentschel; M L Birnstiel
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Authors:  C M Gorman; L F Moffat; B H Howard
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8.  Higher level organization of individual gene transcription and RNA splicing.

Authors:  Y Xing; C V Johnson; P R Dobner; J B Lawrence
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9.  Thymidylate synthetase overproduction in 5-fluorodeoxyuridine-resistant mouse fibroblasts.

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Journal:  Mol Cell Biol       Date:  1982-09       Impact factor: 4.272

10.  Base substitution in an intervening sequence of a beta+-thalassemic human globin gene.

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Journal:  Proc Natl Acad Sci U S A       Date:  1981-04       Impact factor: 11.205

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  16 in total

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2.  Sequence of the polypyrimidine tract of the 3'-terminal 3' splicing signal can affect intron-dependent pre-mRNA processing in vivo.

Authors:  X Liu; J E Mertz
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5.  Comparable processing of beta-lactoglobulin pre-mRNA in cell culture and transgenic mouse models.

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7.  The hepatitis B virus posttranscriptional regulatory element is composed of two subelements.

Authors:  J E Donello; A A Beeche; G J Smith; G R Lucero; T J Hope
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8.  Splicing signals are required for S-phase regulation of the mouse thymidylate synthase gene.

Authors:  Y Ke; J Ash; L F Johnson
Journal:  Mol Cell Biol       Date:  1996-01       Impact factor: 4.272

9.  Genetic variants of CDH13 determine the susceptibility to chronic obstructive pulmonary disease in a Chinese population.

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10.  Isolation of a polyubiquitin promoter and its expression in transgenic potato plants.

Authors:  J E Garbarino; T Oosumi; W R Belknap
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