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控制人类B29基因表达的启动子和5'侧翼序列。

The promoter and 5' flanking sequences controlling human B29 gene expression.

作者信息

Thompson A A, Wood W J, Gilly M J, Damore M A, Omori S A, Wall R

机构信息

Department of Pediatrics, Gwynne Hazen Cherry Memorial Laboratories, Los Angeles, CA, USA.

出版信息

Blood. 1996 Jan 15;87(2):666-73.

PMID:8555489
Abstract

The product of the B-cell-specific B29 gene (B29, Ig beta, CD79b) is essential for Ig-mediated B-cell activation via the B-cell antigen receptor complex (BCR) on human and murine B lymphocytes. To better understand the regulation of this pivotal gene, we have analyzed the human genomic DNA sequence upstream of the B29 ATG start codon for transcriptional control activity. The human B29 gene lacks either a TATA or a CAAT box and transcription is initiated at multiple sites. The minimal promoter of the human B29 gene is contained within a 193-bp region 5' of these multiple start sites. This minimal promoter exhibits B-cell-specific activity and contains SP1, ETS, OCT, and IKAROS/LYF-1 transcription factor motifs. All these motifs are strikingly conserved in sequence and placement relative to the previously characterized murine B29 promoter. Additional upstream gene segments dramatically affected B29 minimal promoter activity. A newly identified motif called the B29 conserved sequence (BCS), found upstream of both human and murine B29 promoters, appears to stimulate B29 transcription through a novel mechanism. A single BCS had little effect either on the minimal B29 promoter or on a heterologous promoter. Instead, the BCS stimulated transcription by counteracting 5' negative regulatory DNA sequences that block the activity of the B29 minimal promoter in its absence. These findings indicate that B29 gene expression is controlled by the complex interplay of positive and negative regulatory elements.

摘要

B细胞特异性B29基因(B29、Igβ、CD79b)的产物对于通过人及小鼠B淋巴细胞上的B细胞抗原受体复合物(BCR)介导的Ig依赖性B细胞活化至关重要。为了更好地理解这个关键基因的调控机制,我们分析了B29 ATG起始密码子上游的人类基因组DNA序列的转录控制活性。人类B29基因既没有TATA框也没有CAAT框,转录起始于多个位点。人类B29基因的最小启动子包含在这些多个起始位点5'端的一个193bp区域内。这个最小启动子表现出B细胞特异性活性,并包含SP1、ETS、OCT和IKAROS/LYF-1转录因子基序。相对于先前鉴定的小鼠B29启动子,所有这些基序在序列和位置上都显著保守。额外的上游基因片段显著影响B29最小启动子的活性。在人类和小鼠B29启动子上游均发现的一个新鉴定的基序,称为B29保守序列(BCS),似乎通过一种新机制刺激B29转录。单个BCS对最小B29启动子或异源启动子几乎没有影响。相反,BCS通过抵消5'负调控DNA序列来刺激转录,这些序列在没有BCS时会阻断B29最小启动子的活性。这些发现表明B29基因表达受正负调控元件复杂相互作用的控制。

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The promoter and 5' flanking sequences controlling human B29 gene expression.控制人类B29基因表达的启动子和5'侧翼序列。
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