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鸡溶菌酶基因5'基质附着区刺激转基因表达及抑制位置效应能力的剖析

Dissection of the ability of the chicken lysozyme gene 5' matrix attachment region to stimulate transgene expression and to dampen position effects.

作者信息

Phi-Van L, Strätling W H

机构信息

Institut für Kleintierforschung, Celle, FR Germany.

出版信息

Biochemistry. 1996 Aug 20;35(33):10735-42. doi: 10.1021/bi9603783.

DOI:10.1021/bi9603783
PMID:8718863
Abstract

The chicken lysozyme gene domain is flanked by nuclear matrix attachment regions (MARs) on each side. We have previously shown that bilaterally flanking 5'MARs in stably transfected artificial genetic units enhance expression of a reporter transgene and dampen position effects of the chromatin structure at the site of integration. The 5' MAR was now dissected into smaller fragments that were monitored for effects on transgene expression in mouse 3T3 cells by a similar assay. Fragments, which contain 1.32 and 1.45 kb and represent the upstream and the downstream half, respectively, of the 5' MAR, retained the ability to stimulate transgene expression as well as the ability to reduce the variation in the level of expression. However, a 452 bp subfragment (H1-HaeII), which still exhibits specific binding to nuclear matrices and contains two high-affinity binding sites for the abundant nuclear matrix protein ARBP, lost both of those abilities. A dimerized 177 bp sequence from fragment H1-HaeII, which also binds selectively to nuclear matrices and includes a duplicated ARBP binding site, was also unable to stimulate reporter gene expression. Furthermore, a 0.65 kb subfragment containing an intrinsically bent sequence did not affect an elevated reporter gene expression and its dampening. Our results show that the ability of MAR fragments to bind to nuclear matrices is not sufficient to enhance and insulate transgene expression in stably transfected cells.

摘要

鸡溶菌酶基因结构域两侧各有一个核基质附着区(MARs)。我们之前已经表明,在稳定转染的人工遗传单位中,两侧的5'MARs可增强报告转基因的表达,并抑制整合位点处染色质结构的位置效应。现在,将5'MAR切割成更小的片段,通过类似的试验监测其对小鼠3T3细胞中转基因表达的影响。分别包含1.32 kb和1.45 kb的片段,分别代表5'MAR的上游和下游半部分,保留了刺激转基因表达的能力以及降低表达水平变化的能力。然而,一个452 bp的亚片段(H1-HaeII),虽然仍表现出与核基质的特异性结合,并且包含两个与丰富的核基质蛋白ARBP的高亲和力结合位点,但却失去了这两种能力。来自片段H1-HaeII的二聚化177 bp序列,也选择性地与核基质结合并包含一个重复的ARBP结合位点,同样无法刺激报告基因的表达。此外,一个包含固有弯曲序列的0.65 kb亚片段不影响报告基因表达的升高及其抑制。我们的结果表明,MAR片段与核基质结合的能力不足以增强和隔离稳定转染细胞中的转基因表达。

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