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一种新的14个碱基对的调控元件对于小鼠β4-半乳糖基转移酶-I在粗线期晚期精母细胞和圆形精子细胞中的体内表达至关重要。

A novel 14-base-pair regulatory element is essential for in vivo expression of murine beta4-galactosyltransferase-I in late pachytene spermatocytes and round spermatids.

作者信息

Charron M, Shaper N L, Rajput B, Shaper J H

机构信息

The Cell Structure and Function Laboratory, The Oncology Center, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21287-8937, USA.

出版信息

Mol Cell Biol. 1999 Aug;19(8):5823-32. doi: 10.1128/MCB.19.8.5823.

Abstract

During murine spermatogenesis, beginning in late pachytene spermatocytes, the beta4-galactosyltransferase-I (beta4GalT-I) gene is transcribed from a male germ cell-specific start site. We had shown previously that a 796-bp genomic fragment that flanks the germ cell start site and contains two putative CRE (cyclic AMP-responsive element)-like motifs directs correct male germ cell expression of the beta-galactosidase reporter gene in late pachytene spermatocytes and round spermatids of transgenic mice (N. L. Shaper, A. Harduin-Lepers, and J. H. Shaper, J. Biol. Chem. 269:25165-25171, 1994). We now report that in vivo expression of beta4GalT-I in developing male germ cells requires an essential and previously undescribed 14-bp regulatory element (5'-GCCGGTTTCCTAGA-3') that is distinct from the two CRE-like sequences. This cis element is located 16 bp upstream of the germ cell-specific start site and binds a male germ cell protein that we have termed TASS-1 (transcriptional activator in late pachytene spermatocytes and round spermatids 1). The presence of the Ets signature binding motif 5'-GGAA-3' on the bottom strand of the TASS-1 sequence (underlined sequence) suggests that TASS-1 is a novel member of the Ets family of transcription factors. Additional transgenic analyses established that an 87-bp genomic fragment containing the TASS-1 regulatory element was sufficient for correct germ cell-specific expression of the beta-galactosidase reporter gene. Furthermore, when the TASS-1 motif was mutated by transversion, within the context of the original 796-bp fragment, transgene expression was reduced 12- to 35-fold in vivo.

摘要

在小鼠精子发生过程中,从粗线期晚期精母细胞开始,β4-半乳糖基转移酶-I(β4GalT-I)基因从雄性生殖细胞特异性起始位点转录。我们之前已经表明,位于生殖细胞起始位点侧翼且包含两个假定的CRE(环磷酸腺苷反应元件)样基序的796 bp基因组片段,可指导β-半乳糖苷酶报告基因在转基因小鼠的粗线期晚期精母细胞和圆形精子细胞中正确地在雄性生殖细胞中表达(N. L. 沙珀、A. 哈迪因-勒佩斯和J. H. 沙珀,《生物化学杂志》269:25165 - 25171,1994年)。我们现在报告,β4GalT-I在发育中的雄性生殖细胞中的体内表达需要一个必需的、以前未描述的14 bp调控元件(5'-GCCGGTTTCCTAGA-3'),该元件与两个CRE样序列不同。这个顺式元件位于生殖细胞特异性起始位点上游16 bp处,并结合一种我们称为TASS-1(粗线期晚期精母细胞和圆形精子细胞中的转录激活因子1)的雄性生殖细胞蛋白。TASS-1序列(下划线序列)底部链上存在Ets特征性结合基序5'-GGAA-3',表明TASS-1是Ets转录因子家族的一个新成员。进一步的转基因分析表明,一个包含TASS-1调控元件的87 bp基因组片段足以使β-半乳糖苷酶报告基因在生殖细胞中特异性正确表达。此外,当在原始796 bp片段的背景下通过颠换使TASS-1基序发生突变时,转基因表达在体内降低了12至35倍。

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