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在低产量菌株的遗传背景下,高产CYP6A2菌株的Cyp6a2等位基因的组成型和巴比妥诱导型表达。

Constitutive and barbital-induced expression of the Cyp6a2 allele of a high producer strain of CYP6A2 in the genetic background of a low producer strain.

作者信息

Dombrowski S M, Krishnan R, Witte M, Maitra S, Diesing C, Waters L C, Ganguly R

机构信息

Department of Biochemistry and Cellular and Molecular Biology, University of Tennessee, Knoxville 37996, USA.

出版信息

Gene. 1998 Oct 9;221(1):69-77. doi: 10.1016/s0378-1119(98)00436-3.

Abstract

The levels of one or more cytochrome P450 (CYP) enzymes and the respective mRNAs are found to be higher in insecticide-resistant insects than in susceptible insects. To understand better how insects regulate the levels of CYPs, we examined the expression of the Cyp6a2 gene in various strains of Drosophila melanogaster. We also took a transgenic approach to understand the molecular mechanisms that are involved in strain variation of Cyp6a2 expression. RNA blot analysis showed that the constitutive expression of Cyp6a2 varies from strain to strain; the level of CYP6A2 mRNA is barely detectable in the underproducer ry506 strain, whereas it is very high in the overproducer 91-R and MHIII-D23 strains. The long terminal repeat (LTR) of mobile element 17.6 that is found in the 3' untranslated region (UTR) of the Cyp6a2 gene of some strains does not appear to have any role on the steady-state CYP6A2 mRNA level. We also found that the Cyp6a2 gene is inducible by barbital in 91-R, ry506 as well as 91-C, which carries an LTR insertion. To examine the genetic background of the underproducer ry506 strain with respect to Cyp6a2 expression, we transformed the ry506 strain with the Cyp6a2 allele of the overproducer 91-R strain (Cyp6a2-91 R) and measured the constitutive and barbital-induced expression of the Cyp6a2-91 R transgene in the transformed flies. The Cyp6a2-91 R transgene carrying 129 bp of DNA upstream of the ATG codon did not show any constitutive or barbital-induced expression in the ry506 host genome. However, transgenes with 1331 and 985 bp upstream DNA showed similar levels of constitutive expression that were higher than that of the endogenous Cyp6a2 gene of the ry506 host strain, but lower than the expression of the same gene in the 91-R strain. Both these transgenes, with 1331 and 985 bp upstream DNA, also showed induction with 0.1 M barbital. DNA sequence analysis revealed that in both 91-R and ry506, the upstream DNA between +1 and -985 bp contains a distal and a proximal group of three potential barbie boxes, i.e. cis-elements that are thought to be involved in barbiturate-mediated induction of CYP genes. Except for four bases located near the distal cluster of barbie boxes and two other bases, the base sequence of the upstream DNA is identical in ry506 and 91-R strains. These results suggest that the underproducer ry506 strain has the trans-regulatory factors to support constitutive and induced expression of the Cyp6a2-91 R allele carrying DNA between -129 and -1331 bp regions. Possible reasons for low constitutive expression of the endogenous Cyp6a2 gene and moderate level of expression of the Cyp6a2-91 R allele in the ry506 genetic background are discussed.

摘要

研究发现,与敏感昆虫相比,抗杀虫剂昆虫体内一种或多种细胞色素P450(CYP)酶及其相应mRNA的水平更高。为了更好地了解昆虫如何调节CYP的水平,我们检测了黑腹果蝇不同品系中Cyp6a2基因的表达。我们还采用转基因方法来了解参与Cyp6a2表达品系变异的分子机制。RNA印迹分析表明,Cyp6a2的组成型表达因品系而异;在低表达品系ry506中几乎检测不到CYP6A2 mRNA的水平,而在高表达品系91-R和MHIII-D23中其水平非常高。在某些品系的Cyp6a2基因3'非翻译区(UTR)中发现的移动元件17.6的长末端重复序列(LTR)似乎对稳态CYP6A2 mRNA水平没有任何作用。我们还发现,在91-R、ry506以及携带LTR插入的91-C中,Cyp6a2基因可被巴比妥诱导。为了研究低表达品系ry506在Cyp6a2表达方面的遗传背景,我们用高表达品系91-R的Cyp6a2等位基因(Cyp6a2-91 R)转化ry506品系,并测量转化果蝇中Cyp6a2-91 R转基因的组成型和巴比妥诱导表达。携带ATG密码子上游129 bp DNA的Cyp6a2-91 R转基因在ry506宿主基因组中未显示任何组成型或巴比妥诱导表达。然而,携带上游1331 bp和985 bp DNA的转基因显示出相似的组成型表达水平,高于ry506宿主品系内源性Cyp6a2基因的表达水平,但低于91-R品系中同一基因的表达水平。这两个携带上游1331 bp和985 bp DNA的转基因也显示出0.1 M巴比妥的诱导作用。DNA序列分析表明,在91-R和ry506中,+1至 -985 bp之间的上游DNA包含一组远端和近端的三个潜在巴比妥盒,即被认为参与巴比妥介导的CYP基因诱导的顺式元件。除了位于巴比妥盒远端簇附近的四个碱基和另外两个碱基外,ry506和91-R品系中上游DNA的碱基序列相同。这些结果表明,低表达品系ry506具有反式调节因子,以支持携带 -129至 -1331 bp区域DNA的Cyp6a2-91 R等位基因的组成型和诱导表达。文中讨论了ry506遗传背景中内源性Cyp6a2基因组成型表达低以及Cyp6a2-91 R等位基因表达水平中等的可能原因。

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