一种来自苔藓植物瀑布藓的新型α-葡萄糖苷酶。

Yamasaki Yoshiki, Nakashima Susumu, Konno Haruyoshi

Research Institute for Bioresources, Okayama University, Okayama, Japan.

Acta Biochim Pol. 2007;54(2):401-6. Epub 2007 May 15.

Scopelophila cataractae is a rare moss that grows on copper-containing soils. S. cataractae protonema was grown on basal MS medium containing copper. A starch-degrading activity was detected in homogenates of the protonema, after successive extraction with phosphate buffer and buffer containing 3 M LiCl. Buffer-soluble extract (BS) and LiCl-soluble extract (LS) readily hydrolyzed amylopectin to liberate only glucose, which shows that alpha-glucosidase (EC 3.2.1.20) in BS and LS hydrolyzed amylopectin. The K(m) value of BS for maltose was 0.427. The K(m) value of BS for malto-oligosaccharide decreased with an increase in the molecular mass of the substrate. The value for maltohexaose was 0.106, which is about four-fold lower than that for maltose. BS was divided into two fractions of alpha-glucosidase (BS-1 and BS-2) by isoelectric focusing. The isoelectric points of these two enzymes were determined to be 4.36 (BS-1) and 5.25 (BS-2) by analytical gel electrofocusing. The two enzymes readily hydrolyzed malto-oligosaccharides. The two enzymes also hydrolyzed amylose, amylopectin and soluble starch at a rate similar to that with maltose. The two enzymes readily hydrolyzed panose to liberate glucose and maltose (1 : 1), and the K(m) value of BS for panose was similar to that for maltotriose, whereas the enzymes hydrolyzed isomaltose only weakly. With regard to substrate specificity, the two enzymes in BS are novel alpha-glucosidases. The two enzymes also hydrolyzed beta-limit dextrin, which has many alpha-1,6-glucosidic linkages near the non-reducing ends, more strongly than maltose, which shows that they do not need a debranching enzyme for starch digestion. The starch-degrading activity of BS was not inhibited by p-chloromercuribenzoic acid or alpha-amylase inhibitor. When amylopectin was treated with BS and LS in phosphate buffer, pH 6.0, glucose, but not glucose-1-phosphate, was detected, showing that the extracts did not contain phosphorylase but did contain an alpha-glucosidase. These results show that alpha-glucosidases should be capable of complete starch digestion by themselves in cells of S. cataractae.

白内障藓是一种生长在含铜土壤上的稀有苔藓。白内障藓原丝体在含铜的基础MS培养基上生长。在用磷酸盐缓冲液和含3M LiCl的缓冲液连续提取后，在原丝体匀浆中检测到淀粉降解活性。缓冲液可溶性提取物（BS）和LiCl可溶性提取物（LS）很容易将支链淀粉水解，只释放出葡萄糖，这表明BS和LS中的α-葡萄糖苷酶（EC 3.2.1.20）水解了支链淀粉。BS对麦芽糖的K（m）值为0.427。BS对麦芽寡糖的K（m）值随着底物分子量的增加而降低。对麦芽六糖的值为0.106，约为麦芽糖值的四分之一。通过等电聚焦将BS分为α-葡萄糖苷酶的两个组分（BS-1和BS-2）。通过分析凝胶电聚焦测定这两种酶的等电点分别为4.36（BS-1）和5.25（BS-2）。这两种酶很容易水解麦芽寡糖。这两种酶还以与麦芽糖相似的速率水解直链淀粉、支链淀粉和可溶性淀粉。这两种酶很容易将潘糖水解，释放出葡萄糖和麦芽糖（1:1），并且BS对潘糖的K（m）值与对麦芽三糖的相似，而这两种酶对异麦芽糖的水解作用较弱。关于底物特异性，BS中的这两种酶是新型α-葡萄糖苷酶。这两种酶还比麦芽糖更强烈地水解β-极限糊精，β-极限糊精在非还原端附近有许多α-1,6-糖苷键，这表明它们在淀粉消化过程中不需要脱支酶。在pH 6.0的磷酸盐缓冲液中，当用BS和LS处理支链淀粉时，检测到葡萄糖，但未检测到葡萄糖-1-磷酸，这表明提取物中不含有磷酸化酶，但含有α-葡萄糖苷酶。这些结果表明，α-葡萄糖苷酶应该能够在白内障藓细胞中自身完成淀粉的消化。