Buck D, Guest J R
Department of Microbiology, University of Sheffield, U.K.
Biochem J. 1989 Jun 15;260(3):737-47. doi: 10.1042/bj2600737.
The succinyl-CoA synthetase of Escherichia coli is encoded by two genes, sucC (beta subunit) and sucD (alpha subunit), which are distal genes in the sucABCD operon. They are expressed from the suc promoter, which also expresses the dehydrogenase and dihydrolipoyl succinyl-transferase subunits of the 2-oxoglutarate dehydrogenase complex. Strategies have now been devised for the site-directed mutagenesis and independent expression of the succinyl-CoA synthetase (alpha 2 beta 2 tetramer) and the individual subunits. These involve (1) subcloning a promoterless sucCD fragment downstream of the lac promoter in M13mp10, and (2) precise splicing of the suc coding regions with the efficient atpE ribosome-binding site and expression from the thermoinducible lambda promoters in the pJLA503 vector. Succinyl-CoA synthetase specific activities were amplified 40-60-fold within 5 h of thermoinduction of the lambda promoters, and the alpha and beta subunits accounted for almost 30% of the protein in supernatant fractions of the cell-free extracts. Site-directed mutagenesis of potential CoA binding-site residues indicated that Trp-43 beta and His-50 beta are essential residues in the beta-subunit, whereas Cys-47 beta could be replaced by serine without inactivating the enzyme. No activity was detected after the histidine residue at the phosphorylation site of the alpha-subunit was replaced by aspartate (His-246 alpha----Asp), but this alteration seemed to have a deleterious effect on the accumulation of the enzyme in cell-free supernatant extracts. The nucleotide sequence of an unidentified gene (g30) that is adjacent to the sucABCD operon was defined by extending the sequence of the citric acid cycle gene cluster by 818 bp to 13379 bp: gltA-sdhCDAB-sucABCD-g30. This gene converges on the suc operon and encodes a product (P30) that contains 230 amino acids (Mr 27,251). Highly significant similarities were detected between the N-terminal region of P30 and those of GENA [the product of another unidentified gene (geneA) located upstream of the aceEF-lpd operon], and GNTR (a putative transcriptional repressor of the gluconate operon of Bacillus subtilis). Possible roles for GENA and P30 as transcriptional regulators of the adjacent operons encoding the pyruvate and 2-oxoglutarate dehydrogenase complexes are discussed.
大肠杆菌的琥珀酰辅酶A合成酶由两个基因sucC(β亚基)和sucD(α亚基)编码,它们是sucABCD操纵子中的远端基因。它们由suc启动子表达,该启动子也表达2-氧代戊二酸脱氢酶复合体的脱氢酶和二氢硫辛酰琥珀酰转移酶亚基。现已设计出用于琥珀酰辅酶A合成酶(α2β2四聚体)和各个亚基的定点诱变及独立表达的策略。这些策略包括:(1)将无启动子的sucCD片段亚克隆到M13mp10中lac启动子的下游;(2)将suc编码区与高效的atpE核糖体结合位点精确拼接,并从pJLA503载体中的热诱导λ启动子进行表达。在λ启动子热诱导5小时内,琥珀酰辅酶A合成酶的比活性提高了40 - 60倍,α和β亚基占无细胞提取物上清液组分中蛋白质的近30%。对潜在辅酶A结合位点残基的定点诱变表明,Trp - 43β和His - 50β是β亚基中的必需残基,而Cys - 47β可被丝氨酸取代而不使酶失活。α亚基磷酸化位点的组氨酸残基被天冬氨酸取代(His - 246α→Asp)后未检测到活性,但这种改变似乎对无细胞上清液提取物中该酶的积累有有害影响。通过将柠檬酸循环基因簇序列延伸818 bp至13379 bp,确定了与sucABCD操纵子相邻的一个未鉴定基因(g30)的核苷酸序列:gltA - sdhCDAB - sucABCD - g30。该基因与suc操纵子汇聚,编码一个含有230个氨基酸(Mr 27251)的产物(P30)。在P30的N端区域与GENA [位于aceEF - lpd操纵子上游的另一个未鉴定基因(geneA)的产物]以及GNTR(枯草芽孢杆菌葡萄糖酸操纵子的一个假定转录阻遏物)的N端区域之间检测到高度显著的相似性。讨论了GENA和P30作为相邻操纵子(编码丙酮酸和2-氧代戊二酸脱氢酶复合体)转录调节因子的可能作用。
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