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A mutant phosphofructokinase produces a futile cycle during gluconeogenesis in Escherichia coli.

机译:突变果糖磷酸激酶在大肠杆菌糖异生过程中产生无效循环。

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摘要

Strains of Escherichia coli bearing different forms of phosphofructokinase were used to assess the occurrence of futile cycling in cell resuspensions supplied with glycerol as gluconeogenic carbon source. A model was used to simulate results of different kinds of experiments for different levels of futile cycle. The main predictions of the model were experimentally confirmed in a strain with a mutant phosphofructokinase-2 (phosphofructokinase-2*) which is not inhibited by MgATP. The intracellular fructose 1, 6-bisphosphate concentration reaches significantly higher levels in the mutant-bearing strain than in strains with either phosphofructokinase-1 or -2. Also, this strain showed a higher rate and level of in vivo radioactive labelling of fructose 1, 6-bisphosphate, from a trace of [U-14C]glucose supplied during gluconeogenesis, indicating higher kinase activity in these conditions. Cell resuspensions of the mutant-bearing strain produced higher levels of radioactively labelled CO2 when supplied with [U-14C]glycerol as the only carbon source. Simultaneously, fewer glycerol carbons were incorporated into HClO4-insoluble macromolecules. Finally, radioactive CO2 output was measured in resuspensions supplied with glycerol as the major carbon source with traces of either [1-14C]glucose or [6-14C]glucose. It was found that, whereas in the strains with either of the wild-type phosphofructokinase isoenzymes, radioactive CO2 output from [1-14C]glucose was higher than with [6-14C]glucose, the reverse is found for the strain with phosphofructokinase-2*. This result also agrees with the corresponding prediction of the model. Using the radioactivity flux rates predicted by the model, an explanation linking the futile cycle to the differential labelling of CO2 is advanced. Finally, on the basis of these results it is proposed that strains bearing phosphofructokinase-2* sustain higher rates of futile cycling during gluconeogenesis than strains bearing either of the wild-type isoforms of phosphofructokinase. The kinetic equations and parameter values used for the model simulations are given in Supplementary Publication SUP 50183 (8 pages), which has been deposited at the British Library Document Supply Centre, Boston Spa, Wetherby, West Yorkshire LS23 7BQ, U.K., from whom copies can be obtained on the terms indicated in Biochem. J. (1997) 321, 8.
机译:带有不同形式的磷酸果糖激酶的大肠杆菌菌株用于评估甘油作为糖原异生碳源提供的细胞重悬中无效循环的发生。使用一个模型来模拟针对不同级别的无效周期的不同类型实验的结果。在带有突变果糖激酶-2(phosphofructokinase-2 *)的菌株中实验证实了该模型的主要预测,该菌株不受MgATP抑制。与携带果糖磷酸激酶-1或-2的菌株相比,携带突变体的菌株中的细胞内果糖1,6-二磷酸酯浓度达到明显更高的水平。而且,该菌株从糖异生过程中提供的痕量[U-14C]葡萄糖中显示出较高的果糖1,6-二磷酸果糖体内放射性标记率和水平,表明在这些条件下具有较高的激酶活性。当携带[U-14C]甘油作为唯一碳源时,携带突变的菌株的细胞重悬会产生更高水平的放射性标记CO2。同时,更少的甘油碳被并入不溶于HClO4的大分子中。最后,在以甘油作为主要碳源的悬浮液中测量了放射性CO2的输出,其中残留有痕量[1-14C]葡萄糖或[6-14C]葡萄糖。发现,在具有野生型磷酸果糖激酶同工酶的菌株中,[1-14C]葡萄糖的放射性CO 2输出高于[6-14C]葡萄糖,而磷酸果糖激酶-的菌株则相反。 2 *。该结果也与模型的相应预测相符。利用模型预测的放射性通量率,提出了将无效循环与CO2差异标记联系起来的解释。最后,基于这些结果,提出带有磷酸果糖激酶-2 *的菌株比带有磷酸果糖激酶的任何野生型同工型的菌株在糖异生期间维持更高的无效循环率。用于模型仿真的动力学方程式和参数值在补充出版物SUP 50183(共8页)中提供,该出版物已存放在英国西约克郡LS23 7BQ韦瑟比市波士顿温泉大学大英图书馆文献供应中心,该书的副本可以按照Biochem中指定的条款获得。 J.(1997)321,8。

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