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人 SHBG mRNA 的翻译受 5'-非编码外显子 1A 和 1B 的选择性调控。

Human SHBG mRNA translation is modulated by alternative 5'-non-coding exons 1A and 1B.

机构信息

Institut de Recerca Hospital Universitari Vall d'Hebrón, Barcelona, Spain.

出版信息

PLoS One. 2010 Nov 4;5(11):e13844. doi: 10.1371/journal.pone.0013844.

Abstract

BACKGROUND

The human sex hormone-binding globulin (SHBG) gene comprises at least 6 different transcription units (TU-1, -1A, -1B, -1C, -1D and -1E), and is regulated by no less than 6 different promoters. The best characterized are TU-1 and TU-1A: TU-1 is responsible for producing plasma SHBG, while TU-1A is transcribed and translated in the testis. Transcription of the recently described TU-1B, -1C, and -1D has been demonstrated in human prostate tissue and prostate cancer cell lines, as well as in other human cell lines such as HeLa, HepG2, HeK 293, CW 9019 and imr 32. However, there are no reported data demonstrating their translation. In the present study, we aimed to determine whether TU-1A and TU-1B are indeed translated in the human prostate and whether 5' UTR exons 1A and 1B differently regulate SHBG translation.

RESULTS

Cis-regulatory elements that could potentially regulate translation were identified within the 5'UTRs of SHBG TU-1A and TU-1B. Although full-length SHBG TU-1A and TU-1B mRNAs were present in prostate cancer cell lines, the endogenous SHBG protein was not detected by western blot in any of them. LNCaP prostate cancer cells transfected with several SHBG constructs containing exons 2 to 8 but lacking the 5'UTR sequence did show SHBG translation, whereas inclusion of the 5'UTR sequences of either exon 1A or 1B caused a dramatic decrease in SHBG protein levels. The molecular weight of SHBG did not vary between cells transfected with constructs with or without the 5'UTR sequence, thus confirming that the first in-frame ATG of exon 2 is the translation start site of TU-1A and TU-1B.

CONCLUSIONS

The use of alternative SHBG first exons 1A and 1B differentially inhibits translation from the ATG situated in exon 2, which codes for methionine 30 of transcripts that begin with the exon 1 sequence.

摘要

背景

人类性激素结合球蛋白 (SHBG) 基因至少包含 6 种不同的转录单元 (TU-1、-1A、-1B、-1C、-1D 和 -1E),并受不少于 6 种不同启动子的调控。其中 TU-1 和 TU-1A 研究得最为透彻:TU-1 负责产生血浆 SHBG,而 TU-1A 则在睾丸中转录和翻译。最近描述的 TU-1B、-1C 和 -1D 的转录已在人前列腺组织和前列腺癌细胞系中得到证实,以及在其他细胞系如 HeLa、HepG2、HeK 293、CW 9019 和 imr 32 中得到证实。然而,目前还没有报道表明它们的翻译情况。在本研究中,我们旨在确定 TU-1A 和 TU-1B 是否确实在人前列腺中进行翻译,以及 5'UTR 外显子 1A 和 1B 是否不同地调节 SHBG 翻译。

结果

在 SHBG TU-1A 和 TU-1B 的 5'UTR 中发现了可能调节翻译的顺式调节元件。虽然全长 SHBG TU-1A 和 TU-1B mRNA 存在于前列腺癌细胞系中,但在任何一种细胞系中都未通过 Western blot 检测到内源性 SHBG 蛋白。转染了包含外显子 2 到 8 但缺乏 5'UTR 序列的几种 SHBG 构建体的 LNCaP 前列腺癌细胞确实显示出 SHBG 翻译,而包含外显子 1A 或 1B 的 5'UTR 序列会导致 SHBG 蛋白水平显著降低。转染带有或不带有 5'UTR 序列的构建体的细胞中 SHBG 的分子量没有变化,因此证实外显子 2 中的第一个框内 ATG 是 TU-1A 和 TU-1B 的翻译起始位点。

结论

使用替代的 SHBG 第一个外显子 1A 和 1B 会差异抑制从位于外显子 2 中的 ATG 开始的翻译,该外显子 2 编码从外显子 1 序列开始的转录物的甲硫氨酸 30。

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