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大肠杆菌中的葡萄糖代谢以及醛缩酶量增加的影响。

Glucose metabolism in Escherichia coli and the effect of increased amount of aldolase.

作者信息

Babul J, Clifton D, Kretschmer M, Fraenkel D G

机构信息

Department of Microbiology and Molecular Genetics, Harvard Medical School, Boston, Massachusetts 02115.

出版信息

Biochemistry. 1993 May 4;32(17):4685-92. doi: 10.1021/bi00068a029.

Abstract

We present a comparative study of Escherichia coli with normal and increased amounts of fructose-1,6-bisphosphate aldolase. Most experiments employed a resting cell system involving a high cell density (so as to obtain the soluble pool by direct extraction) and anaerobic incubation in the presence of chloramphenicol. Glucose use is linear with time with a rate ca. half of that in growth, fermentation is almost quantitative, and metabolite concentrations reach a quasi steady state. Increased amount of aldolase had little effect on glucose flux; fructose-1,6-P2 concentration decreased by ca. one-third, and the extent of equilibration of its two halves, measured by a dismutation procedure on samples taken during metabolism of [6-14C]glucose, increased from 0.33 [(cpm in C1-3)/(cpm in C1-6)] to 0.43. Using the simplest model, that increased amount of aldolase does not perturb net flux or later metabolites, together with the steady-state rate equations for aldolase and triose-P isomerase, we show that the results with resting cells fit with the extra enzyme being fully active, and do not necessitate special assumptions concerning a glycolytic complex, metabolite compartmentation, or secondary mechanisms assuring high metabolite concentration. However, the fit does require that the measured Vmax values substantially underestimate the actual ones. Calculation also shows that the forms of the predicted curves--and hence the fit with experimental data--of fructose-1,6-P2 concentration and labeling as a function of the amount of aldolase are highly dependent on glyceraldehyde-3-P concentration but independent of the kinetic parameters of aldolase.

摘要

我们对具有正常量和增加量果糖-1,6-二磷酸醛缩酶的大肠杆菌进行了一项比较研究。大多数实验采用静止细胞系统,该系统具有高细胞密度(以便通过直接提取获得可溶性池),并在氯霉素存在下进行厌氧培养。葡萄糖的利用与时间呈线性关系,速率约为生长时的一半,发酵几乎是定量的,代谢物浓度达到准稳态。醛缩酶量的增加对葡萄糖通量影响不大;果糖-1,6-P2浓度降低了约三分之一,通过对[6-14C]葡萄糖代谢过程中采集的样品进行歧化程序测量,其两半部分的平衡程度从0.33[(C1-3中的cpm)/(C1-6中的cpm)]增加到0.43。使用最简单的模型,即醛缩酶量的增加不会干扰净通量或后续代谢物,结合醛缩酶和磷酸丙糖异构酶的稳态速率方程,我们表明静止细胞的结果符合额外的酶完全有活性的情况,并且不需要关于糖酵解复合物、代谢物区室化或确保高代谢物浓度的二级机制的特殊假设。然而,这种拟合确实要求测量的Vmax值大大低估了实际值。计算还表明,果糖-1,​​6-P2浓度和标记作为醛缩酶量的函数的预测曲线形式(因此与实验数据的拟合)高度依赖于甘油醛-3-P浓度,但与醛缩酶的动力学参数无关。

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