Kawabata Atsufumi, Kanke Toru, Yonezawa Daiki, Ishiki Tsuyoshi, Saka Masako, Kabeya Mototsugu, Sekiguchi Fumiko, Kubo Satoko, Kuroda Ryotaro, Iwaki Masahiro, Katsura Kousaku, Plevin Robin
Division of Physiology and Pathophysiology, School of Pharmaceutical Sciences, Kinki University, 3-4-1 Kowakae, Higashi-Osaka 577-8502, Japan.
J Pharmacol Exp Ther. 2004 Jun;309(3):1098-107. doi: 10.1124/jpet.103.061010. Epub 2004 Feb 19.
To develop potent and metabolically stable agonists for protease-activated receptor-2 (PAR-2), we prepared 2-furoylated (2f) derivatives of native PAR-2-activating peptides, 2f-LIGKV-OH, 2f-LIGRL-OH, 2f-LIGKV-NH(2), and 2f-LIGRL-NH(2), and systematically evaluated their activity in PAR-2-responsive cell lines and tissues. In both HCT-15 cells and NCTC2544 cells overexpressing PAR-2, all furoylated peptides increased cytosolic Ca(2+) levels with a greater potency than the corresponding native peptides, although a similar maximum response was recorded. The absolute potency of each peptide was greater in NCTC2544, possibly due to a higher level of receptor expression. Furthermore, the difference in potency between the 2-furoylated peptides and the native peptides was enhanced when evaluated in the rat superior mesenteric artery and further increased when measuring PAR-2-mediated salivation in ddY mice in vivo. The potency of 2f-LIGRL-NH(2), the most powerful peptide, relative to SLIGKV-OH, was about 100 in the cultured cell Ca(2+) signaling assays, 517 in the vasorelaxation assay, and 1100 in the salivation assay. Amastatin, an aminopeptidase inhibitor, augmented salivation caused by native peptides, but not furoylated peptides. The PAR-2-activating peptides, including the furoylated derivatives, also produced salivation in the wild-type C57BL/6 mice, but not the PAR-2-deficient mice. Our data thus demonstrate that substitution of the N-terminal serine with a furoyl group in native PAR-2-activating peptides dramatically enhances the agonistic activity and decreases degradation by aminopeptidase, leading to development of 2f-LIGRL-NH(2), the most potent peptide. Furthermore, the data from PAR-2-deficient mice provide ultimate evidence for involvement of PAR-2 in salivation and the selective nature of the 2-furoylated peptides.
为开发用于蛋白酶激活受体-2(PAR-2)的强效且代谢稳定的激动剂,我们制备了天然PAR-2激活肽的2-呋喃甲酰化(2f)衍生物,即2f-LIGKV-OH、2f-LIGRL-OH、2f-LIGKV-NH₂和2f-LIGRL-NH₂,并系统评估了它们在PAR-2反应性细胞系和组织中的活性。在过表达PAR-2的HCT-15细胞和NCTC2544细胞中,所有呋喃甲酰化肽均能提高胞质Ca²⁺水平,且效力高于相应的天然肽,不过记录到的最大反应相似。每种肽在NCTC2544中的绝对效力更高,这可能是由于受体表达水平更高。此外,在大鼠肠系膜上动脉中评估时,2-呋喃甲酰化肽与天然肽之间的效力差异增大,而在体内测量ddY小鼠中PAR-2介导的唾液分泌时,该差异进一步增加。在培养细胞Ca²⁺信号测定中,最强效的肽2f-LIGRL-NH₂相对于SLIGKV-OH的效力约为100,在血管舒张测定中为517,在唾液分泌测定中为1100。氨肽酶抑制剂抑肽酶增强了天然肽引起的唾液分泌,但未增强呋喃甲酰化肽引起的唾液分泌。包括呋喃甲酰化衍生物在内的PAR-2激活肽在野生型C57BL/6小鼠中也能引起唾液分泌,但在PAR-2缺陷小鼠中则不能。因此,我们的数据表明,在天然PAR-2激活肽中将N端丝氨酸替换为呋喃甲酰基可显著增强激动活性并减少氨肽酶的降解,从而开发出了最有效的肽2f-LIGRL-NH₂。此外,来自PAR-2缺陷小鼠的数据为PAR-2参与唾液分泌以及2-呋喃甲酰化肽的选择性提供了最终证据。
