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在人单核细胞系U-937中表达的42种不同的Krüppel相关锌指蛋白的cDNA克隆的分离。

Isolation of cDNA clones for 42 different Krüppel-related zinc finger proteins expressed in the human monoblast cell line U-937.

作者信息

Abrink M, Aveskogh M, Hellman L

机构信息

Department of Immunology, University of Uppsala, The Biomedical Centre, Sweden.

出版信息

DNA Cell Biol. 1995 Feb;14(2):125-36. doi: 10.1089/dna.1995.14.125.

DOI:10.1089/dna.1995.14.125
PMID:7865130
Abstract

To study the complexity and structural characteristics of zinc finger proteins expressed during human hematopoiesis and to isolate novel regulators of blood cell development, a degenerate oligonucleotide probe specific for a consensus zinc finger peptide domain was used to isolate 63 cDNA clones for Krüppel-related zinc finger genes from the human monoblast cell line U-937. By extensive nucleotide sequence and Northern blot analysis, these cDNA clones were found to originate from approximately 42 different genes (HZF 1-42) of which only 8 have previously been described. Northern blot analysis showed that a majority of these genes were expressed at comparable levels in U-937 and HeLa cells. The large number of individual genes represented among the 63 clones and their apparent non-cell-type-specific expression suggest that the majority of the Krüppel-related zinc finger genes are likely to be expressed in most human tissues. In contrast, some of the genes displayed a restricted expression pattern, indicating that they represent potential regulators of monocyte differentiation or proliferation. Detailed structural analysis of the first 12 cDNAs (HZF 1-10) and a partial characterization of HZF 11-42 revealed that a common feature of human Krüppel-related zinc finger proteins is the presence of tandem arrays of zinc fingers ranging in number from 3 to over 20 that are preferentially located in the carboxy-terminal regions of the proteins. In addition, several novel KRAB-containing zinc finger genes and a novel conserved sequence element were identified.

摘要

为了研究人类造血过程中表达的锌指蛋白的复杂性和结构特征,并分离血细胞发育的新型调节因子,使用针对共有锌指肽结构域的简并寡核苷酸探针,从人单核细胞系U-937中分离出63个与Krüppel相关的锌指基因的cDNA克隆。通过广泛的核苷酸序列和Northern印迹分析,发现这些cDNA克隆源自大约42个不同的基因(HZF 1-42),其中只有8个先前已有描述。Northern印迹分析表明,这些基因中的大多数在U-937和HeLa细胞中以相当的水平表达。63个克隆中代表的大量单个基因及其明显的非细胞类型特异性表达表明,大多数与Krüppel相关的锌指基因可能在大多数人类组织中表达。相比之下,一些基因表现出受限的表达模式,表明它们代表单核细胞分化或增殖的潜在调节因子。对前12个cDNA(HZF 1-10)的详细结构分析以及HZF 11-42的部分特征表明,人类与Krüppel相关的锌指蛋白的一个共同特征是存在数量从3到超过20个不等的锌指串联阵列,这些阵列优先位于蛋白质的羧基末端区域。此外,还鉴定了几个新的含KRAB的锌指基因和一个新的保守序列元件。

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