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用可水解唾液酸的酶处理豚鼠结肠带后其收缩性及钙结合的变化

Changes in contractility and calcium binding of guinea pig taenia coli by treatment with enzymes which hydrolyze sialic acid.

作者信息

Ishiyama Y, Yabu H, Miyazaki E

出版信息

Jpn J Physiol. 1975;25(6):719-32. doi: 10.2170/jjphysiol.25.719.

Abstract

The effects of neuraminidase and phospholipase C on the contractility and the Ca++ -binding of guinea pig taenia coli were investigated. Potassium contracture or histamine-induced contracture of taenia coli was inhibited by treatment with neuraminidase, though acetylcholine-induced contracture was not. Treatment with phospholipase C markedly inhibited the contracture induced by isotonic potassium, histamine or acetylcholine. By treatment with neuraminidase for 4 hr, about 40 mumol/100 mg wer wt of sialic acid was released from taenia coli. This corresponded to two-fifths of total content of sialic acid. By treatment with phospholipase C for 2 hr, a similar amount of sialic acid to that produced by neuraminidase treatment was released. The Scarchard plot of Ca++-binding was a biphasic pattern indicating the presence of two types ofthe Ca++ -binding site with different affinity constants. Neuraminidase produced a 57% decrease in the amount of bound Ca++. The Scatchard plot of Ca++ -binding changed to a monophasic pattern indicating the disapperance of thel ow affinity Ca++ -binding site. Phospholipase C caused a 59% decrease of bound Ca++. The Scatchard plot also indicated the disappearance of the low affinity Ca++ -binding site. From these results, we speculated that sialicacid residue of surface membrane of the muscle cell was first site in the Ca++ -influx mechanism.

摘要

研究了神经氨酸酶和磷脂酶C对豚鼠结肠带收缩性及钙离子结合的影响。用神经氨酸酶处理可抑制结肠带的钾离子挛缩或组胺诱导的挛缩,但对乙酰胆碱诱导的挛缩无抑制作用。用磷脂酶C处理可显著抑制等渗钾、组胺或乙酰胆碱诱导的挛缩。用神经氨酸酶处理4小时后,结肠带释放出约40μmol/100mg湿重的唾液酸,这相当于唾液酸总含量的五分之二。用磷脂酶C处理2小时后,释放出的唾液酸量与神经氨酸酶处理产生的量相似。钙离子结合的Scatchard图呈双相模式,表明存在两种具有不同亲和常数的钙离子结合位点。神经氨酸酶使结合钙离子的量减少了57%。钙离子结合的Scatchard图变为单相模式,表明低亲和力钙离子结合位点消失。磷脂酶C使结合钙离子减少了59%。Scatchard图也表明低亲和力钙离子结合位点消失。根据这些结果,我们推测肌细胞膜表面的唾液酸残基是钙离子内流机制的首要位点。

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