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来自黄化甜菜(Beta vulgaris L. var. lutea)毛状根的谷氨酰胺合成酶同工酶、寡聚体和亚基。

Glutamine synthetase isoenzymes, oligomers and subunits from hairy roots of Beta vulgaris L. var. lutea.

作者信息

Mäck G

机构信息

Albrecht-von-Haller-Institut für Pflanzenwissenschaften, Universität Göttingen, Germany.

出版信息

Planta. 1998 May;205(1):113-20. doi: 10.1007/s004250050302.

DOI:10.1007/s004250050302
PMID:9599808
Abstract

A cytosolic and a plastidic isoenzyme of glutamine synthetase (GS; EC 6.3.1.2) were separated from hairy roots of Beta vulgaris L. var. lutea. The predominant activity was that of cytosolic GS 1; the relative proportion of plastidic GS 2 activity changed, however, depending on the growth conditions. Maximum activity of both isoenzymes was measured after growth with NO3- as the major N-source. Growth with NH4+ as the sole N-source or growth in constant darkness resulted in a significant decrease in GS 1 activity, whereas GS 2 activity was much less effected and thus contributed as much as 25% of total root GS activity. The isoenzymes GS 1 and GS 2 were active both in the octameric and tetrameric states. Both oligomers of GS 2 and octameric GS 1 were active under all growth conditions applied whereas tetrameric GS 1 was not active when the roots were grown under light-dark changes with NO3- as the major N-source. The molecular masses of the subunits were identical for both isoenzymes. Glutamine synthetase 1 was composed of up to four different 38-kDa subunits and two different 41-kDa subunits; GS 2 was assembled from one type of 38-kDa subunit and one type of 41-kDa subunit. The GS 2 subunits were most probably identical to two of the GS 1 subunits. The subunit composition of GS 1, but not of GS 2, changed depending on the growth conditions of the roots. Changes in GS 1 subunit composition were correlated with changes in GS 1 activity. The different growth conditions induced the specific assembly of different GS 1 isoenzymes which could, however, not be separated by anion-exchange chromatography but became evident only after two-dimensional sodium dodecyl sulfate-polyacrylamide gel electrophoresis.

摘要

从甜菜(Beta vulgaris L. var. lutea)的毛状根中分离出谷氨酰胺合成酶(GS;EC 6.3.1.2)的一种胞质同工酶和一种质体同工酶。主要活性是胞质GS 1的活性;然而,质体GS 2活性的相对比例会根据生长条件而变化。以NO3-作为主要氮源生长后,两种同工酶的活性均达到最大值。以NH4+作为唯一氮源生长或在持续黑暗中生长会导致GS 1活性显著降低,而GS 2活性受影响较小,因此占总根GS活性的比例高达25%。同工酶GS 1和GS 2在八聚体和四聚体状态下均有活性。GS 2的两种寡聚体和八聚体GS 1在所有应用的生长条件下均有活性,而当根在以NO3-作为主要氮源的光暗变化条件下生长时,四聚体GS 1无活性。两种同工酶的亚基分子量相同。谷氨酰胺合成酶1由多达四种不同的38 kDa亚基和两种不同的41 kDa亚基组成;GS 2由一种类型的38 kDa亚基和一种类型的41 kDa亚基组装而成。GS 2亚基很可能与GS 1亚基中的两个相同。GS 1的亚基组成会根据根的生长条件而变化,但GS 2不会。GS 1亚基组成的变化与GS 1活性的变化相关。不同的生长条件诱导了不同GS 1同工酶的特异性组装,然而,这些同工酶不能通过阴离子交换色谱分离,只有在二维十二烷基硫酸钠-聚丙烯酰胺凝胶电泳后才变得明显。

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