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An Accounting of Horseradish Peroxidase Isozymes Associated with the Cell Wall and Evidence that Peroxidase Does Not Contain Hydroxyproline

机译:与细胞壁相关的辣根过氧化物酶同工酶的核算和过氧化物酶不含羟脯氨酸的证据

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摘要

Isopycnic equilibrium centrifugation techniques were used to determine whether any horseradish (Amoracia lapathifolia) peroxidase isozymes were associated with hydroxyproline containing moieties. Purified peroxidase, horseradish root extracts, and peroxidase isozymes released from horseradish root cell walls were tested. In no case could any peak of peroxidase activity be found to band with hydroxyproline.A fluorimetric method for measurement of peroxidase activity was used to determine quantitatively the amount of total peroxidase located on horseradish root cell walls. Twenty per cent of the total peroxidase is found in the cell wall fraction after extraction; 93% of this cell wall associated peroxidase can be removed by washing with 2 m NaCl. Some peroxidase isozymes released by salt washing are not found in the cytoplasmic extract. This indicates that not all of the ionically bound peroxidase represents cytoplasmic contamination. The 1.4% of the total peroxidase activity can thus be considered tightly bound to the cell wall. Of this portion, 75% can be solubilized by treatment with a cellulase preparation. One isozyme is released which was not present in the original cytoplasmic extract.
机译:用等渗平衡离心技术确定辣根(Amoracia lapathifolia)过氧化物酶同工酶是否与含羟脯氨酸的部分相关。测试了从辣根根细胞壁释放的纯化的过氧化物酶,辣根提取物和过氧化物酶同工酶。在任何情况下都不会发现任何羟脯氨酸过氧化物酶的活性峰。用荧光法测定过氧化物酶的活性,定量测定辣根根细胞壁上总过氧化物酶的量。提取后在细胞壁部分发现总过氧化物酶的百分之二十;通过用2 m NaCl洗涤可以除去93%的与细胞壁相关的过氧化物酶。通过盐洗释放的一些过氧化物酶同工酶在细胞质提取物中未发现。这表明并非所有离子结合的过氧化物酶都代表细胞质污染。因此,总过氧化物酶活性的1.4%被认为与细胞壁紧密结合。在这部分中,可以通过用纤维素酶制剂处理来溶解75%。释放出一种不存在于原始细胞质提取物中的同工酶。

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