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小麦胚芽天冬氨酸转氨甲酰酶。纯化及冷不稳定性。

Wheat-germ aspartate transcarbamoylase. Purification and cold-lability.

作者信息

Grayson J E, Yon R J, Butterworth P J

出版信息

Biochem J. 1979 Nov 1;183(2):239-45. doi: 10.1042/bj1830239.

Abstract
  1. Aspartate transcarbamoylase was purified approx. 3000-fold from wheat (Triticum vulgare) germ in 15-20% yield. The product has a specific activity of 14 mumol/min per mg of protein and is approx. 90% pure. The purification scheme includes the use of biospecific "imphilyte" chromatography as described by Yon [Biochem.J.(1977) 161, 233-237]. The enzyme was passed successively through columns of CPAD [N-(3-carboxypropionyl)aminodecyl]-Sepharose in the absence and presence respectively of the ligands UMP and L-aspartate. In the second passage the enzyme was specifically displaced away from impurities with which it co-migrated in the first passage. These two steps contributed a factor of 80 to the overall purification. 2. The enzyme is slowly inactivated on dilution at 0 degrees C and pH 7.0, the inactivation being partially reversible. A detailed investigation of the temperature- and pH-dependence of the cold-inactivation suggested that it was initiated by the perturbation of the pKa values of groups with a moderately high and positive heat of ionization, which were tentatively identified as histidine residues. These findings support a new concept of cold-lability proposed by Bock, Gilbert & Frieden [Biochem. Biophys. Res. Commun. (1975) 66, 564-569].
摘要
  1. 天冬氨酸转氨甲酰酶从小麦(普通小麦)胚芽中纯化得到,纯化倍数约为3000倍,产率为15 - 20%。该产物的比活性为每毫克蛋白质14微摩尔/分钟,纯度约为90%。纯化方案包括使用如Yon所述的生物特异性“两性电解质”色谱法[《生物化学杂志》(1977年)161卷,233 - 237页]。酶先后通过CPAD [N -(3 - 羧基丙酰基)氨基癸基]-琼脂糖柱,分别在不存在和存在配体UMP和L - 天冬氨酸的情况下。在第二次通过时,酶被特异性地从第一次通过时与其共迁移的杂质中置换出来。这两个步骤对整体纯化的贡献系数为80。2. 该酶在0℃和pH 7.0下稀释时会缓慢失活,失活部分可逆。对冷失活的温度和pH依赖性的详细研究表明,它是由电离热适中且为正的基团的pKa值受到扰动引发的,这些基团初步鉴定为组氨酸残基。这些发现支持了Bock、Gilbert和Frieden提出的冷不稳定性新概念[《生物化学与生物物理研究通讯》(1975年)66卷,564 - 569页]。

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