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大肠杆菌中S-腺苷甲硫氨酸合成酶的调控

Regulation of S-adenosylmethionine synthetase in Escherichia coli.

作者信息

Holloway C T, Greene R C, Su C H

出版信息

J Bacteriol. 1970 Nov;104(2):734-47. doi: 10.1128/jb.104.2.734-747.1970.

Abstract

Addition of methionine to the growth medium of Escherichia coli K-12 leads to a reduction in the specific activity of S-adenosylmethionine (SAM) synthetase. Thus the enzyme appears to be repressible rather than inducible. Mutant strains (probably metJ(-)) are constitutive for SAM synthetase as well as for the methionine biosynthetic enzymes, suggesting that the regulatory systems for these enzymes have at least some elements in common. Cells grown to stationary phase in complete medium, which have low specific activities of the enzymes, were routinely used for derepression experiments. The lag in growth and derepression when these cells are incubated in minimal medium is shortened by threonine. Ethionine, norleucine, and alpha-methylmethionine are poor substrates or nonsubstrates for SAM synthetase and are ineffective repressors. Selenomethionine, a better substrate for SAM synthetase than methionine, is also slightly more effective at repression than methionine. Although SAM is considered to be a likely candidate for the corepressor in the control of the methionine biosynthetic enzymes, addition of SAM to the growth medium does not cause repression. Measurement of SAM uptake shows that too little is taken into the cells to have a significant effect, even if it were active in the control system.

摘要

向大肠杆菌K-12的生长培养基中添加甲硫氨酸会导致S-腺苷甲硫氨酸(SAM)合成酶的比活性降低。因此,该酶似乎是可阻遏的,而非可诱导的。突变菌株(可能是metJ(-))对SAM合成酶以及甲硫氨酸生物合成酶呈组成型表达,这表明这些酶的调节系统至少有一些共同的元件。在完全培养基中生长至稳定期的细胞,其酶的比活性较低,通常用于去阻遏实验。当这些细胞在基本培养基中培养时,苏氨酸可缩短其生长和去阻遏的延迟时间。乙硫氨酸、正亮氨酸和α-甲基甲硫氨酸是SAM合成酶的劣质底物或非底物,且是无效的阻遏物。硒代甲硫氨酸是SAM合成酶比甲硫氨酸更好的底物,在阻遏方面也比甲硫氨酸稍有效。尽管SAM被认为是甲硫氨酸生物合成酶控制中可能的辅阻遏物候选者,但向生长培养基中添加SAM不会导致阻遏。SAM摄取量的测量表明,即使它在控制系统中起作用,进入细胞的量也太少,不会产生显著影响。

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