Pinko C, Margosiak S A, Vanderpool D, Gutowski J C, Condon B, Kan C C
Molecular Biology/Biochemistry Group, Agouron Pharmaceuticals, Inc., San Diego, California 92121, USA.
J Biol Chem. 1995 Oct 6;270(40):23634-40. doi: 10.1074/jbc.270.40.23634.
We report here the production of active recombinant single-chain human cytomegalovirus protease in Escherichia coli and development of a continuous assay for this protease. In order to produce the human cytomegalovirus (HCMV) protease for structural studies and accurate kinetic analysis, mutation of alanine 143 at an internal cleavage site was introduced to prevent auto-proteolysis. The resulting soluble 29-kDa A143Q protease was purified to homogeneity as a stable single-chain protein by hydrophobic interaction and ionic-exchange chromatography. The in vivo protein substrate, assembly protein precursor, was also expressed and purified for activity studies. To develop a continuous protease assay, fluorescent synthetic peptide substrates similar to the cleavage sequence P5 to P5' of the maturation site containing anthranilic acid and nitrotyrosine as a resonance energy transfer donor-acceptor pair were designed. Purified HCMV A143Q protease cleaved the recombinant assembly protein precursor with Km and kcat values of 3.0 +/- 1.0 microM and 13.3 +/- 1.6 min-1. The Km for peptide substrates is at least 45-fold higher than for the natural protein substrate, but the kcat values are similar. A sensitive assay was developed using fluorescent peptide substrates, which can detect nM HCMV protease activity.
我们在此报告在大肠杆菌中生产活性重组单链人巨细胞病毒蛋白酶以及开发针对该蛋白酶的连续检测方法。为了生产用于结构研究和精确动力学分析的人巨细胞病毒(HCMV)蛋白酶,在内部切割位点引入丙氨酸143突变以防止自催化裂解。通过疏水相互作用和离子交换色谱法将所得的可溶性29 kDa A143Q蛋白酶纯化为均一的稳定单链蛋白。体内蛋白底物装配蛋白前体也被表达和纯化用于活性研究。为了开发连续蛋白酶检测方法,设计了类似于成熟位点切割序列P5至P5'的荧光合成肽底物,其包含邻氨基苯甲酸和硝基酪氨酸作为共振能量转移供体-受体对。纯化的HCMV A143Q蛋白酶切割重组装配蛋白前体,其Km和kcat值分别为3.0±1.0μM和13.3±1.6 min-1。肽底物的Km比天然蛋白底物至少高45倍,但kcat值相似。使用荧光肽底物开发了一种灵敏的检测方法,该方法可以检测纳摩尔级的HCMV蛋白酶活性。
