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Derepression of the glyoxylate cycle in mutants of Neurospora crassa accelerated for growth on acetate

机译:Neurospora Crassa突变体中甘油酯循环的DEREPLACE,加速乙酸盐生长

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Two spontaneous allelic mutations have been isolated with the unusual semi-dominant phenotype of faster-than-wild-type growth on acetate as sole carbon source. The mutants were designated Aag-1 (accelerated acetate growth) and mapped on linkage group II. Upon re-isolation of both the Aag-1 alleles from repeated back-crosses to wild-type, between 1 and 6% of the progeny were found to be acu (acetate non-utilizing) mutants. Ten of these were selected for heterokaryon complementation analysis with known acu mutants; nine proved to be new alleles of acu-5 (deficient in acetyl-CoA synthetase), and one was a new acetate non-utilizing class, designated acu-14. Although the Aag-1 mutants clearly have no acetate-growth-related enzyme deficiencies, they did exhibit significant constitutive enzyme levels for acetyl-CoA synthetase and the glyoxylate cycle enzymes (isocitrate lyase and malate synthase) on the non-inducing carbon source, sucrose. The derepression was restricted to these enzymes, as representative enzymes from other carbon-assimilatory pathways remained repressed and subject to carbon catabolite repression. Northern blot analysis of the mRNA levels of acetyl-CoA synthetase and the glyoxylate cycle enzymes from the mutants demonstrated the derepression to occur at the level of transcription. These data suggest that the physiological explanation for the accelerated acetate growth phenotype lies in the standing levels of the acetate-assimilatory enzymes, which enable the mutants to forgo some of the normal time required for adaption to growth on acetate.
机译:两种自发等位基因突变已被分离出不寻常的半导性表型,其乙酸盐较快的型生长速度较快,作为唯一的碳源。突变体被指定为AAG-1(加速乙酸盐生长)并映射在连杆族II上。在再分离从重复背交到野生型的AAG-1等位基因,发现1至6%的后代是ACU(醋酸酸不使用)突变体。其中十分之一被选为已知的ACU突变体的异质官官能互补分析;九九被证明是ACU-5的新等位基因(缺乏乙酰-CoA合成酶),一种是新的醋酸甲酸盐非利用阶级,指定ACU-14。虽然AAG-1突变体显然没有醋酸生长相关的酶缺陷,但它们确实在非诱导碳源,蔗糖上表现出乙酰-CoA合成酶和乙氧基化酶循环酶(异柠檬酸裂解酶和雄性合成酶)的显着组成酶水平。 DEREMENTIONTS仅限于这些酶,因为来自其他碳 - 同化途径的代表性酶仍然被压抑,受碳分子抑制的影响。来自突变体的乙酰-CoA合成酶的mRNA水平的Northern印迹分析和来自突变体的乙氧基化循环酶在转录水平上表明了DERELAGESS。这些数据表明,加速醋酸酯生长表型的生理解释位于醋酸酯 - 同化酶的站立水平,使得突变体能够用于适应乙酸盐生长所需的一些正常时间。

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