Tanco Sebastian, Zhang Xin, Morano Cain, Avilés Francesc Xavier, Lorenzo Julia, Fricker Lloyd D
Departament de Bioquimica, Institut de Biotecnologia i de Biomedicina, Universitat Autonoma de Barcelona, Bellaterra, Barcelona, Spain.
J Biol Chem. 2010 Jun 11;285(24):18385-96. doi: 10.1074/jbc.M109.060350. Epub 2010 Apr 12.
CPA4 (carboxypeptidase A4) is a member of the metallocarboxypeptidase family. CPA4 was originally found in a screen of mRNAs up-regulated by sodium butyrate-induced differentiation of cancer cells. Further studies suggested a relation between CPA4 and prostate cancer aggressiveness. In the present study, we determined that CPA4 is secreted from cells as a soluble proenzyme (pro-CPA4) that can be activated by endoproteases, such as trypsin. Three complementary approaches were used to study the substrate specificity of CPA4; kinetic analysis was performed using a new series of chromogenic substrates and some biologically relevant peptides, the cleavage of synthetic peptides was tested individually, and the cleavage of a mixture of >100 mouse brain peptides was examined using a quantitative peptidomics mass spectrometry-based approach. CPA4 was able to cleave hydrophobic C-terminal residues with a preference for Phe, Leu, Ile, Met, Tyr, and Val. However, not all peptides with C-terminal hydrophobic residues were cleaved, indicating the importance of additional residues within the peptide. Aliphatic, aromatic, and basic residues in the P1 position have a positive influence on the cleavage specificity. In contrast, acidic residues, Pro, and Gly have a negative influence in the P1 position. Some of the peptides identified as CPA4 substrates (such as neurotensin, granins, and opioid peptides) have been previously shown to function in cell proliferation and differentiation, potentially explaining the link between CPA4 and cancer aggressiveness. Taken together, these studies suggest that CPA4 functions in neuropeptide processing and regulation in the extracellular environment.
羧肽酶A4(CPA4)是金属羧肽酶家族的一员。CPA4最初是在对丁酸钠诱导癌细胞分化后上调的mRNA进行筛选时发现的。进一步的研究表明CPA4与前列腺癌侵袭性之间存在关联。在本研究中,我们确定CPA4作为一种可溶性酶原(pro-CPA4)从细胞中分泌出来,它可以被诸如胰蛋白酶等内切蛋白酶激活。我们采用了三种互补的方法来研究CPA4的底物特异性;使用一系列新的生色底物和一些具有生物学相关性的肽进行动力学分析,单独测试合成肽的切割情况,并使用基于定量肽组学质谱的方法检测100多种小鼠脑肽混合物的切割情况。CPA4能够切割疏水性C末端残基,优先选择苯丙氨酸、亮氨酸、异亮氨酸、甲硫氨酸、酪氨酸和缬氨酸。然而,并非所有具有C末端疏水性残基的肽都会被切割,这表明肽内其他残基的重要性。P1位置的脂肪族、芳香族和碱性残基对切割特异性有积极影响。相比之下,酸性残基、脯氨酸和甘氨酸在P1位置有负面影响。一些被鉴定为CPA4底物的肽(如神经降压素、嗜铬粒蛋白和阿片肽)先前已被证明在细胞增殖和分化中起作用,这可能解释了CPA4与癌症侵袭性之间的联系。综上所述,这些研究表明CPA4在细胞外环境中的神经肽加工和调节中发挥作用。