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在一个基因不稳定的黑腹果蝇品系中,从叉状和切割位点精确切除反转录转座子吉普赛。

Precise excision of the retrotransposon gypsy from the forked and cut loci in a genetically unstable D. melanogaster strain.

作者信息

Kuzin A B, Lyubomirskaya N V, Khudaibergenova B M, Ilyin Y V, Kim A I

机构信息

V.A. Engelhardt Institute of Molecular Biology, Academy of Sciences of Russia, Moscow.

出版信息

Nucleic Acids Res. 1994 Nov 11;22(22):4641-5. doi: 10.1093/nar/22.22.4641.

Abstract

The genetically unstable Mutator Strain of D. melanogaster is characterised by a high frequency of spontaneous mutations and their reversions. Three forked mutants were obtained independently and several reversions arose spontaneously with frequency of 10(-3)-10(-4). The sites of integration and excision of the gypsy retrotransposon were analysed by Southern blot analysis and sequencing of PCR fragments. In all cases gypsy had inserted at the end of the third exon of the major transcript of the forked gene, causing the duplication of TCCA target sequence. All the reversions resulted from precise excision of the gypsy. A double mutant containing ct6 and f1, caused by gypsy insertions into untranslated regions of the corresponding genes, was constructed. Two spontaneous ct6f+ revertants as well as one ct+f1 revertant were obtained from this line. Sequence analysis of gypsy integration and excision sites revealed that in all cases gypsy excision was also precise. These experiments constitute the first demonstration of precise excision of LTR-containing elements from their host genomes.

摘要

黑腹果蝇的遗传不稳定突变体菌株的特征是自发突变及其回复突变的频率很高。独立获得了三个叉状突变体,并且自发出现了几个回复突变体,频率为10(-3)-10(-4)。通过Southern印迹分析和PCR片段测序分析了gypsy逆转座子的整合和切除位点。在所有情况下,gypsy都插入到叉状基因主要转录本的第三个外显子末端,导致TCCA靶序列重复。所有回复突变都是由gypsy的精确切除引起的。构建了一个由gypsy插入相应基因的非翻译区引起的包含ct6和f1的双突变体。从该品系中获得了两个自发的ct6f +回复突变体以及一个ct + f1回复突变体。gypsy整合和切除位点的序列分析表明,在所有情况下,gypsy的切除也是精确的。这些实验首次证明了含LTR元件从其宿主基因组中的精确切除。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1d4a/308512/c9b19d4fbb26/nar00046-0101-a.jpg

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