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小鼠肝脏和肾脏中磷脂酶B活性的电子显微镜证实

Electron microscopic demonstration of phospholipase B activity in the liver and the kidney of the mouse.

作者信息

Nagata T, Iwadare N

出版信息

Histochemistry. 1984;80(2):149-52. doi: 10.1007/BF00679989.

Abstract

A method has been developed for electron microscopic histochemical demonstration of phospholipase B, (lecithinase B, E C 3.1.1.5, lysolecithin acyl hydrolase), which hydrolyzes alpha- and beta-positions of phospholipids in mouse liver, kidney and adrenal tissues. Tissues either fixed in cold 1% paraformaldehyde or unfixed were cut into 40 micrometers frozen sections and were incubated at 37 degrees C in a medium at pH 6.6 or 4.5 containing 2 microM lysolecithin and 0.25 mM CaCl2 for 20 min. The fatty acids liberated by enzymatic hydrolysis were trapped as calcium precipitate and were converted to lead precipitate by treatment with lead nitrate. The reaction products were observed by electron microscopy to be localized on the end of the smooth endoplasmic reticulum at pH 6.6 and in lysosomes and lipid droplets at pH 4.5. It is concluded that the products showed the localization of phospholipase B activity.

摘要

已开发出一种用于电子显微镜组织化学显示磷脂酶B(卵磷脂酶B,EC 3.1.1.5,溶血卵磷脂酰基水解酶)的方法,该酶可水解小鼠肝脏、肾脏和肾上腺组织中磷脂的α和β位。固定于冷1%多聚甲醛的组织或未固定的组织被切成40微米的冰冻切片,并在37℃下于pH 6.6或4.5的培养基中孵育20分钟,该培养基含有2微摩尔溶血卵磷脂和0.25毫摩尔氯化钙。酶促水解释放的脂肪酸以钙沉淀形式捕获,并用硝酸铅处理后转化为铅沉淀。通过电子显微镜观察,反应产物在pH 6.6时定位于光滑内质网末端,在pH 4.5时定位于溶酶体和脂滴中。结论是产物显示了磷脂酶B活性的定位。

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