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U1小核RNA变体在家蚕细胞中共存。

U1 snRNA variants coexist in Bombyx mori cells.

作者信息

Gao J P, Herrera R J

机构信息

Department of Biological Sciences, Florida International University, Miami 33199, USA.

出版信息

Insect Mol Biol. 1995 Aug;4(3):193-202. doi: 10.1111/j.1365-2583.1995.tb00025.x.

Abstract

Evidence for at least four U1 snRNA variants were obtained from a U1 cDNA library using U1 snRNA from Bombyx mori BmN cells in culture. Sequence analysis of thirty cDNA clones showed that: (1) the nucleotide changes are in the hairpin structures I, II and III; (2) the majority of the base changes in stem structures between a posterior silk gland (PSG) U1 RNA and the BmN U1 clones, as well as among the BmN U1 clones, are compensatory; (3) although the base differences between PSG U1 and BmN U1 clones, and among the BmN U1 clones, are not the same, they are located in similar positions in moderately conserved sites, frequently at the bases of loops; (4) when comparing the PSG U1 with the BmN U1 clones, twelve out of nineteen stem differences generate stronger pairing resulting in a more stable hairpin II in the BmN U1 clones; and (5) the Sm and 70K proteins binding site sequences are highly conserved among these U1 clones. Although a comparison of sequences changes associated with U1 isoforms from different species indicate that there are no common base changes with the B. mori U1 clones reported here, similarities in the multitude and location of base differences in hairpins I, II and III are observed in mouse and/or Xenopus. It is possible that U1 variants like the ones reported here play a role in alternative pre-mRNA splicing by way of different RNA-protein factor interactions.

摘要

利用培养的家蚕BmN细胞中的U1 snRNA,从U1 cDNA文库中获得了至少四种U1 snRNA变体的证据。对30个cDNA克隆的序列分析表明:(1)核苷酸变化存在于发夹结构I、II和III中;(2)后部丝腺(PSG)U1 RNA与BmN U1克隆之间以及BmN U1克隆之间茎结构中的大多数碱基变化是互补的;(3)尽管PSG U1与BmN U1克隆之间以及BmN U1克隆之间的碱基差异不同,但它们位于中度保守位点的相似位置,经常位于环的基部;(4)将PSG U1与BmN U1克隆进行比较时,19个茎差异中有12个产生更强的配对,导致BmN U1克隆中的发夹II更稳定;(5)这些U1克隆中Sm和70K蛋白结合位点序列高度保守。尽管对来自不同物种的与U1亚型相关的序列变化进行比较表明,与本文报道的家蚕U1克隆没有共同的碱基变化,但在小鼠和/或非洲爪蟾中观察到发夹I、II和III中碱基差异的数量和位置存在相似性。本文报道的这种U1变体可能通过不同的RNA-蛋白质因子相互作用在可变前体mRNA剪接中发挥作用。

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