Schád Eva, Farkas Attila, Jékely Gáspár, Tompa Peter, Friedrich Peter
Institute of Enzymology, Biological Research Center, Hungarian Academy of Sciences, H-1518 Budapest, P.O. Box 7, Hungary.
Biochem J. 2002 Mar 1;362(Pt 2):383-8. doi: 10.1042/0264-6021:3620383.
Typical calpains are heterodimeric cysteine proteases which have distinct large catalytic subunits (80 kDa) but share a common small regulatory subunit (30 kDa; css1). Here we report the identification, cloning and characterization of a novel human small subunit (css2) encoded by an intronless gene, capns2, located on chromosome 16. This new protein displays 73% sequence identity within the Ca(2+)-binding region but lacks two oligo-Gly stretches characteristic of the N-terminal domain of the conventional small subunit. css2 appears to be the functional equivalent of the conventional small subunit in vitro in that it helps the large subunit fold into the active conformation of similar Ca(2+) sensitivity when the two proteins are co-expressed in Escherichia coli. The purification of various chimaeric rat 80 kDa-human css2 constructs, on the other hand, shows that css2 binds the large subunit much more weakly than css1. Further, it does not undergo the autolytic conversion typical of the classical small subunit. The expression of this protein in vivo, as assessed from its appearance in expressed sequence tag clones, is rather limited, making it an example of a tissue-specific, rather than ubiquitous, small subunit.
典型的钙蛋白酶是异二聚体半胱氨酸蛋白酶,具有不同的大催化亚基(80 kDa),但共享一个共同的小调节亚基(30 kDa;css1)。在此,我们报告了一种由位于16号染色体上的无内含子基因capns2编码的新型人类小亚基(css2)的鉴定、克隆和特征。这种新蛋白质在Ca(2+)结合区域内显示出73%的序列同一性,但缺乏传统小亚基N端结构域特有的两个寡聚甘氨酸序列。在体外,css2似乎等同于传统的小亚基,因为当这两种蛋白质在大肠杆菌中共表达时,它有助于大亚基折叠成具有相似Ca(2+)敏感性的活性构象。另一方面,各种嵌合大鼠80 kDa-人类css2构建体的纯化表明,css2与大亚基的结合比css1弱得多。此外,它不会经历典型的经典小亚基的自溶转化。根据其在表达序列标签克隆中的出现情况评估,该蛋白质在体内的表达相当有限,使其成为组织特异性而非普遍存在的小亚基的一个例子。
