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Subcellular Location of O-Acetylserine Sulfhydrylase Isoenzymes in Cell Cultures and Plant Tissues of Datura innoxia Mill.

机译:曼陀罗无毒工厂的细胞培养和植物组织中O-乙酰丝氨酸巯基化酶同工酶的亚细胞定位。

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摘要

O-Acetylserine sulfhydrylase (OASS; EC 4.2.99.8) catalyzes the formation of L-cysteine from O-acetylserine and inorganic sulfide. Three OASS isoenzymes that differ in molecular mass and subunit structure are present in shoot and root tissues and in cadmium-resistant and cadmium-susceptible cell cultures of Datura innoxia Mill. Different OASS forms predominate in leaves, roots, and suspension-cell cultures. To determine the subcellular location of the OASS isoenzymes, purified mitochondria, chloroplasts, and cytosolic fractions from protoplasts were obtained. The isoenzymes are compartmentalized in D. innoxia cells, with a different isoenzyme predominant in the chloroplast, cytosol, and mitochondria, suggesting that they serve different functions in the plant cell. The chloroplast form is most abundant in green leaves and leaf protoplasts. The cytosolic form is most abundant in roots and cell cultures. A mitochondrial form is abundant in cell cultures, but is a minor form in leaves or roots. Cadmium-tolerant cell cultures contain 1.8 times as much constitutive OASS activity as the wild-type cell line, and 2.9 times more than the cadmium-hypersensitive cell line. This may facilitate rapid production of glutathione and metal-binding phytochelatins when these cultures are exposed to cadmium.
机译:O-乙酰丝氨酸巯基化酶(OASS; EC 4.2.99.8)催化由O-乙酰丝氨酸和无机硫化物形成L-半胱氨酸。曼陀罗无毒工厂的枝条和根部组织以及抗镉和对镉敏感的细胞培养物中均存在三种分子量和亚基结构不同的OASS同工酶。在叶片,根和悬浮细胞培养物中,不同的OASS形式占主导。为了确定OASS同工酶的亚细胞位置,从原生质体中获得了纯化的线粒体,叶绿体和胞质级分。这些同工酶在D.nonoxia细胞中区分开,在叶绿体,胞质溶胶和线粒体中主要存在不同的同工酶,这表明它们在植物细胞中发挥着不同的功能。叶绿体形式在绿叶和叶原生质体中含量最高。胞质形式在根和细胞培养物中最丰富。线粒体形式在细胞培养物中含量很高,但在叶或根中是次要形式。耐受镉的细胞培养物的组成型OASS活性是野生型细胞系的1.8倍,是对镉过敏的细胞系的2.9倍。当这些培养物暴露于镉时,这可能有助于快速生产谷胱甘肽和与金属结合的植物螯合物。

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