Cohn P D, Emanuel P D, Bozdech M J
Blood. 1987 Jun;69(6):1574-9.
Nonspecific esterase (NSE) is used to identify normal and leukemic mononuclear phagocytes cytochemically. It can be demonstrated by the hydrolysis of alpha-naphthyl acetate or butyrate. NSE from leukapheresed leukemic monocytes were extracted with several types of detergent and grouped into two isoelectric point (pl) categories based on the ease of solubility: pl 5.7-6.3 (8 bands) greater than or equal to pl 6.6-7.6 (6 bands). Normal monocytes yielded only the pl 5.7-6.3 isozymes. Isozymes from both leukemic and normal monocytes were inhibited similarly by sodium fluoride, pH less than 4.7, and a serine active site inhibitor. All isozymes were bound by Sepharose-concanavalin A (Con-A) and displayed similar substrate preferences and pH v activity slopes. Under the conditions of detergent solubilization, the smallest mol wt species retaining enzymatic activity was 50 +/- 5 kd. Despite these similarities, the isozymes of pl 5.7 through 6.3 and pl greater than 6.3 exhibited different degrees or types of inhibition by phenylmethylsulfonyl fluoride (PMSF), resistance to heat and antigenic character. Thus, the esterase isozymes represent two families of glycoproteins, both of them probable cell surface enzymes, resembling classical liver carboxyl or B-esterases (EC 3.1.1 1).
非特异性酯酶(NSE)用于通过细胞化学方法鉴定正常和白血病单核吞噬细胞。它可通过α-萘乙酸或丁酸的水解来显示。从白细胞去除的白血病单核细胞中提取的NSE用几种类型的去污剂处理,并根据溶解性的难易程度分为两个等电点(pl)类别:pl 5.7 - 6.3(8条带)大于或等于pl 6.6 - 7.6(6条带)。正常单核细胞仅产生pl 5.7 - 6.3同工酶。白血病单核细胞和正常单核细胞的同工酶受到氟化钠、pH小于4.7以及丝氨酸活性位点抑制剂的类似抑制。所有同工酶都与琼脂糖-伴刀豆球蛋白A(Con - A)结合,并表现出相似的底物偏好和pH - v活性斜率。在去污剂溶解的条件下,保留酶活性的最小分子量物种为50±5 kd。尽管有这些相似之处,但pl 5.7至6.3和pl大于6.3的同工酶在苯甲基磺酰氟(PMSF)抑制程度或类型、耐热性和抗原特性方面表现不同。因此,酯酶同工酶代表两个糖蛋白家族,它们可能都是细胞表面酶,类似于经典的肝脏羧基或B酯酶(EC 3.1.1 1)。
