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从大鼠舌浆液腺中纯化舌淀粉酶以及大鼠舌淀粉酶和舌脂肪酶的特性研究

Purification of lingual amylase from serous glands of rat tongue and characterization of rat lingual amylase and lingual lipase.

作者信息

Field R B, Spielman A I, Hand A R

机构信息

National Institute of Dental Research, National Institutes of Health, Bethesda, Maryland 20892.

出版信息

J Dent Res. 1989 Feb;68(2):139-45. doi: 10.1177/00220345890680020801.

Abstract

Lingual amylase and lingual lipase, two digestive enzymes that are secreted from lingual serous glands (von Ebner's), were simultaneously purified from rat lingual serous glands with hydrophobic chromatography used as the final step. This method, previously developed for the purification of lingual lipase, includes homogenization of rat lingual serous glands, 100,000 g centrifugation, ammonium sulfate precipitation of proteins, and extraction of lipids with acetone at -20 degrees C, followed by hydrophobic chromatography on ethyl agarose or Agethane. Amylase was eluted after the elution of proteins that did not interact with the hydrophobic gel at pH 6.3. Lingual lipase was eluted with a solution containing micelles of taurodeoxycholate, monoolein, and oleic acid. Analysis of each of the purified enzymes by SDS-polyacrylamide gel electrophoresis revealed one band at Mr = 59,000 for amylase and one band at Mr = 51,000 for lingual lipase. Isoelectric focusing of amylase indicated a strong band at pI = 5.0 and two very faint bands at pI = 4.9 and 4.8, possibly isozymes or deamidated protein. Amino acid and hexosamine analyses were performed on the enzymes after electroelution from SDS-polyacrylamide gels. Both lingual lipase and lingual amylase had a high content of dicarboxylic (free and amide) amino acids. For lingual lipase and lingual amylase, the % molar ratios of aspartic acid/asparagine were 15.35 and 15.10, and the % molar ratios of glutamic acid/glutamine were 7.07 and 7.20, respectively. Lingual amylase was very similar to rat parotid, pancreatic, and mouse salivary amylases, except that it contained more proline (11.03% molar ratio).(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

舌淀粉酶和舌脂肪酶是由舌浆液腺(冯·埃布纳腺)分泌的两种消化酶,最终通过疏水色谱法从大鼠舌浆液腺中同时纯化得到。这种先前用于纯化舌脂肪酶的方法,包括大鼠舌浆液腺的匀浆、100,000g离心、蛋白质的硫酸铵沉淀以及在-20℃下用丙酮提取脂质,随后在乙基琼脂糖或Agethane上进行疏水色谱。在pH 6.3时,与疏水凝胶不相互作用的蛋白质洗脱后,淀粉酶被洗脱。舌脂肪酶用含有牛磺脱氧胆酸盐、单油酸甘油酯和油酸胶束的溶液洗脱。通过SDS-聚丙烯酰胺凝胶电泳对每种纯化酶进行分析,结果显示淀粉酶在Mr = 59,000处有一条带,舌脂肪酶在Mr = 51,000处有一条带。淀粉酶的等电聚焦表明在pI = 5.0处有一条强带,在pI = 4.9和4.8处有两条非常淡的带,可能是同工酶或脱酰胺蛋白。从SDS-聚丙烯酰胺凝胶上电洗脱后,对酶进行了氨基酸和己糖胺分析。舌脂肪酶和舌淀粉酶都含有高含量的二羧酸(游离和酰胺)氨基酸。对于舌脂肪酶和舌淀粉酶,天冬氨酸/天冬酰胺的摩尔百分比分别为15.35和15.10,谷氨酸/谷氨酰胺的摩尔百分比分别为7.07和7.20。舌淀粉酶与大鼠腮腺、胰腺和小鼠唾液淀粉酶非常相似,只是它含有更多的脯氨酸(摩尔比为11.03%)。(摘要截短于250字)

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