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仓鼠CAD基因cDNA的构建及其在确定天冬氨酸转氨甲酰酶结构域中的应用。

Construction of a cDNA to the hamster CAD gene and its application toward defining the domain for aspartate transcarbamylase.

作者信息

Shigesada K, Stark G R, Maley J A, Niswander L A, Davidson J N

出版信息

Mol Cell Biol. 1985 Jul;5(7):1735-42. doi: 10.1128/mcb.5.7.1735-1742.1985.

Abstract

cDNA complementary to hamster mRNA encoding the CAD protein, a multifunctional protein which carries the first three enzymes of pyrimidine biosynthesis, was constructed. The longest of these recombinants (pCAD142) covers 82% of the 7.9-kilobase mRNA. Portions of the cDNA were excised and replaced by a lac promoter-operator-initiation codon segment. The resultant plasmids were transfected into an Escherichia coli mutant defective in aspartate transcarbamylase, the second enzyme of the pathway. Complementation of the bacterial defect was observed with as little as 2.2 kilobases of cDNA sequence, corresponding to the 3' region of the mRNA. DNA sequencing in this region of the hamster cDNA reveals stretches which are highly homologous to the E. coli gene for the catalytic subunit of aspartate transcarbamylase; other stretches show no homology. The highly conserved regions probably reflect areas of protein structure critical to catalysis, while the nonconserved regions may reflect differences between the quaternary structures of E. coli and mammalian aspartate transcarbamylases, one such difference being that the bacterial enzyme in its native form is allosterically regulated and the mammalian enzyme is not.

摘要

构建了与仓鼠编码CAD蛋白的mRNA互补的cDNA,CAD蛋白是一种多功能蛋白,它携带嘧啶生物合成的前三种酶。这些重组体中最长的(pCAD142)覆盖了7.9千碱基mRNA的82%。切除cDNA的部分片段,并用一个乳糖启动子-操纵子-起始密码子片段进行替换。将所得质粒转染到天冬氨酸转氨甲酰酶(该途径的第二种酶)有缺陷的大肠杆菌突变体中。观察到仅用2.2千碱基的cDNA序列(对应于mRNA的3'区域)就能补充细菌的缺陷。仓鼠cDNA这一区域的DNA测序揭示了与大肠杆菌天冬氨酸转氨甲酰酶催化亚基基因高度同源的片段;其他片段则没有同源性。高度保守的区域可能反映了对催化至关重要的蛋白质结构区域,而非保守区域可能反映了大肠杆菌和哺乳动物天冬氨酸转氨甲酰酶四级结构的差异,其中一个差异是细菌酶以天然形式存在时受到别构调节,而哺乳动物酶则不受此调节。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5c3f/367292/f0597270bf29/molcellb00103-0202-a.jpg

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