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人源甲酰肽受体编码基因的克隆。启动子区域的特征分析及多态性表达证据。

Cloning of the gene coding for a human receptor for formyl peptides. Characterization of a promoter region and evidence for polymorphic expression.

作者信息

Perez H D, Holmes R, Kelly E, McClary J, Chou Q, Andrews W H

机构信息

Department of Medicine, University of California, San Francisco 94143.

出版信息

Biochemistry. 1992 Nov 24;31(46):11595-9. doi: 10.1021/bi00161a044.

DOI:10.1021/bi00161a044
PMID:1445895
Abstract

Recently we reported that, in HL-60 cells, transcription of the formyl peptide receptor (FPR) gene can be up- and downregulated by agents that induce differentiation of HL-60 cells into neutrophils. To begin studying the mechanisms involved in regulation of FPR gene expression, we cloned two human cDNAs and the gene coding for FPR. The genomic clone (pINF14) contained a 14.5-kb insert. A 2.7-kb EcoRI fragment was obtained from pINF14 that hybridized with an FPR open reading frame probe. The EcoRI fragment was sequenced and found to contain an intronless FPR open reading frame. Sequence alignment of the EcoRI genomic fragment with the FPR cDNA revealed that the first 31 bases of 5' untranslated FPR cDNA were not represented in the genomic fragment. Furthermore, a splicing consensus sequence was present in the genomic fragment at the site of divergence with the cDNA sequence. Restriction mapping and Southern blot analysis identified a 121-bp fragment that contained the sequence corresponding to the first 31 bases of 5' untranslated FPR cDNA. An additional (previously undescribed) 15-bp cDNA sequence in the 5' end of FPR were identified using an anchored polymerase chain reaction. This sequence was also contained in the genomic 121-bp fragment. This 121-bp fragment was located 5.2 kb (intron) upstream of the FPR open reading frame. It contained an unusual TATA box and displayed transcriptional activity in vitro and in vivo. Potential binding sites for AP-1 and glucocorticoid receptor were identified upstream of the putative TATA box.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

最近我们报道,在HL-60细胞中,甲酰肽受体(FPR)基因的转录可被诱导HL-60细胞分化为中性粒细胞的试剂上调和下调。为了开始研究FPR基因表达调控的机制,我们克隆了两个人类cDNA和编码FPR的基因。基因组克隆(pINF14)包含一个14.5 kb的插入片段。从pINF14获得了一个2.7 kb的EcoRI片段,它与FPR开放阅读框探针杂交。对该EcoRI片段进行测序,发现其包含一个无内含子的FPR开放阅读框。EcoRI基因组片段与FPR cDNA的序列比对显示,FPR cDNA 5'非翻译区的前31个碱基在基因组片段中未出现。此外,在基因组片段中与cDNA序列不同的位点存在一个剪接共有序列。限制性酶切图谱分析和Southern印迹分析鉴定出一个121 bp的片段,其包含与FPR cDNA 5'非翻译区前31个碱基对应的序列。使用锚定聚合酶链反应在FPR的5'端鉴定出一个额外的(以前未描述的)15 bp cDNA序列。该序列也包含在基因组121 bp片段中。这个121 bp的片段位于FPR开放阅读框上游5.2 kb(内含子)处。它包含一个不寻常的TATA盒,并在体外和体内显示出转录活性。在假定的TATA盒上游鉴定出了AP-1和糖皮质激素受体的潜在结合位点。(摘要截短于250字)

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