Department of Biomedical Sciences, Creighton University School of Medicine, 2500 California Plaza, Omaha, NE 68178, USA.
Peptides. 2009 Dec;30(12):2263-7. doi: 10.1016/j.peptides.2009.09.012. Epub 2009 Sep 15.
Gastrin-17-Gly (G17-Gly) has been shown to bind to non-CCK nanomolar and micromolar affinity sites on DLD-1 and HT-29 human colonic carcinoma cells and to stimulate cellular proliferation. However, in previous studies, we showed that C-terminal truncation of the gastrin-17 (G17) to the G17 analog G17(1-12) and then to G17(1-6)-NH(2) did not remove the ability to bind to DLD-1 cells or to activate proliferation. This implies that residues and/or structural motifs required for bioactivity at these receptors rest in the N-terminal region of G17. In this work, radioligand binding studies conducted with further C-terminally truncated analogs revealed that sequences as short as G17(1-4) still bind to a single receptor with micromolar affinity. Additionally, cell proliferation assays showed that G17(1-12) stimulates proliferation of DLD-1 cells, as of HT-29 cells, but the sequences shorter than G17(1-6)-NH(2), including non-amidated G17(1-6), were incapable of stimulating proliferation. These observations indicate that the tetrapeptide pGlu-Gly-Pro-Trp is the minimum N-terminal sequence for binding to the probable growth-promoting site on DLD-1 cells. Since analogs shorter than G17(1-6) are able to bind the receptor, these peptides may be of use for developing selective antagonists.
胃泌素-17-甘氨酸(G17-Gly)已被证明能与 DLD-1 和 HT-29 人结肠癌细胞上的非 CCK 纳摩尔和微摩尔亲和力结合位点结合,并刺激细胞增殖。然而,在之前的研究中,我们表明,胃泌素-17(G17)的 C 端截短为 G17 类似物 G17(1-12),然后为 G17(1-6)-NH(2),并没有去除与 DLD-1 细胞结合或激活增殖的能力。这意味着在这些受体上具有生物活性所需的残基和/或结构基序位于 G17 的 N 端区域。在这项工作中,用进一步 C 端截短的类似物进行的放射性配体结合研究表明,短至 G17(1-4)的序列仍然与单个具有微摩尔亲和力的受体结合。此外,细胞增殖实验表明,G17(1-12)刺激 DLD-1 细胞的增殖,如同 HT-29 细胞一样,但短于 G17(1-6)-NH(2)的序列,包括非酰胺化的 G17(1-6),不能刺激增殖。这些观察结果表明,四肽 pGlu-Gly-Pro-Trp 是与 DLD-1 细胞上可能的促生长位点结合的最小 N 端序列。由于短于 G17(1-6)的类似物能够结合受体,这些肽可能用于开发选择性拮抗剂。
