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酿酒酵母中L-色氨酸的转运

Transport of L-tryptophan in Saccharomyces cerevisiae.

作者信息

Kotyk A, Dvoráková M

机构信息

Department of Membrane Transport, Czechoslovak Academy of Sciences, Prague.

出版信息

Folia Microbiol (Praha). 1990;35(3):209-17. doi: 10.1007/BF02820487.

Abstract

In addition to the general amino acid transport system (GAP) of S. cerevisiae L-tryptophan is transported by another system with approximately 25% capacity of GAP, with a KT of 0.41 +/- 0.08 mmol/L and with a similar specificity as GAP (lower inhibition by Met, Pro, Ser, Thr and 2-aminoisobutyric acid; greater inhibition by Glu and His). The pH optimum of this system is at 5.0-5.5, activation energy above the transition point (20 degrees C) was 20 kJ/mol, below the transition point 55 kJ/mol. The transport by this system was virtually unidirectional, efflux amounting to at most 10% into a tryptophan-free medium. The transport itself was blocked by 2,4-dinitrophenol, antimycin A and uranyl nitrate. The system was synthesized de novo during preincubation with glucose = fructose greater than trehalose greater than ethanol within 30 min, and was degraded with a half-time of 15 min in the absence of further synthesis. The accumulation ratios of L-tryptophan in gap1 mutants were concentration-dependent (200:1 at 1 mumol L-Trp/L, 4:1 at 2.5 mmol L-Trp/L) and decreased with increasing suspension density from 200:1 to 5:1 (for 10 mumol L-Trp/L). The involvement of hydrogen ions in the uptake was clearly demonstrated by the effect of D2O even if it could not be established by either shifts of pHout or membrane depolarization.

摘要

除了酿酒酵母的一般氨基酸转运系统(GAP)外,L-色氨酸还可通过另一个转运系统进行转运,该系统的转运能力约为GAP的25%,转运常数(KT)为0.41±0.08 mmol/L,特异性与GAP相似(对甲硫氨酸、脯氨酸、丝氨酸、苏氨酸和2-氨基异丁酸的抑制作用较低;对谷氨酸和组氨酸的抑制作用较强)。该系统的最适pH值为5.0 - 5.5,高于转变点(20℃)时的活化能为20 kJ/mol,低于转变点时为55 kJ/mol。该系统的转运几乎是单向的,向无色氨酸培养基中的外流量最多为10%。2,4-二硝基苯酚、抗霉素A和硝酸铀酰可阻断该转运过程。在与葡萄糖=果糖>海藻糖>乙醇预孵育30分钟内,该系统可从头合成,在无进一步合成的情况下,其降解半衰期为15分钟。在gap1突变体中,L-色氨酸的积累率呈浓度依赖性(在1 μmol L-色氨酸/L时为200:1,在2.5 mmol L-色氨酸/L时为4:1),并且随着悬浮密度从200:1增加到5:1(对于10 μmol L-色氨酸/L)而降低。即使无法通过细胞外pH值变化或膜去极化来确定,但重水的作用清楚地证明了氢离子参与了色氨酸的摄取过程。

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