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一种影响前体mRNA剪接和核内前体mRNA滞留的条件性U5小核RNA突变将SSD1/SRK1鉴定为一种普遍的剪接突变体抑制因子。

A conditional U5 snRNA mutation affecting pre-mRNA splicing and nuclear pre-mRNA retention identifies SSD1/SRK1 as a general splicing mutant suppressor.

作者信息

Luukkonen B G, Séraphin B

机构信息

European Molecular Biology Laboratory, Meyerhofstrasse 1, D-69117 Heidelberg, Germany.

出版信息

Nucleic Acids Res. 1999 Sep 1;27(17):3455-65. doi: 10.1093/nar/27.17.3455.

Abstract

A combination of point mutations disrupting both stem 1 and stem 2 of U5 snRNA (U5AI) was found to confer a thermosensitive phenotype in vivo. In a strain expressing U5AI, pre-mRNA splicing was blocked before the first step through an inability of the mutant U5 snRNA to efficiently associate with the U4/U6 di-snRNP. Formation of early splicing complexes was not affected in extracts prepared from U5 snRNA mutant cells, while the capacity of these extracts to splice a pre-mRNA in vitro was greatly diminished. In addition, significant levels of a translation product derived from intron containing pre-mRNAs could be detected in vivo. The SSD1/SRK1 gene was identified as a multi-copy suppressor of the U5AI snRNA mutant. Single copy expression of SSD1/SRK1 was sufficient to suppress the thermosensitive phenotype, and high copy expression partially suppressed the splicing and U4/U6.U5 tri-snRNP assembly pheno-types. SSD1/SRK1 also suppressed thermosensitive mutations in the Prp18p and U1-70K proteins, while inhibiting growth of the cold sensitive U1-4U snRNA mutant at 30 degrees C. Thus we have identified SSD1/SRK1 as a general suppressor of splicing mutants.

摘要

研究发现,破坏U5 snRNA(U5AI)茎1和茎2的点突变组合在体内可导致温度敏感表型。在表达U5AI的菌株中,由于突变的U5 snRNA无法有效地与U4/U6双snRNP结合,前体mRNA剪接在第一步之前就被阻断。从U5 snRNA突变细胞制备的提取物中,早期剪接复合体的形成不受影响,而这些提取物在体外剪接前体mRNA的能力则大大降低。此外,在体内可检测到来自含内含子前体mRNA的显著水平的翻译产物。SSD1/SRK1基因被鉴定为U5AI snRNA突变体的多拷贝抑制子。SSD1/SRK1的单拷贝表达足以抑制温度敏感表型,高拷贝表达则部分抑制剪接和U4/U6·U5三snRNP组装表型。SSD1/SRK1还抑制Prp18p和U1-70K蛋白中的温度敏感突变,同时在30℃时抑制冷敏感U1-4U snRNA突变体的生长。因此,我们已将SSD1/SRK1鉴定为剪接突变体的一般抑制子。

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