Hill D J, Strutt B, Arany E, Zaina S, Coukell S, Graham C F
Lawson Research Institute, St. Joseph's Health Center, London, Ontario, Canada.
Endocrinology. 2000 Mar;141(3):1151-7. doi: 10.1210/endo.141.3.7354.
In rats, a proportion of pancreatic beta-cells are deleted by apoptosis in the second week of postnatal life and replaced by endocrine cell neogenesis from pancreatic ductal epithelium. This coincides with a reduction in pancreatic insulin-like growth factor II (IGF-II) expression, and IGF-II has been shown to act as a beta-cell survival factor in vitro. To examine whether IGF-II regulates beta-cell apoptosis in vivo, an IGF-II transgenic mouse model was used in which mouse IGF-II is overexpressed in skin, gut, and uterus driven by a keratin promoter, so that circulating IGF-II is retained postnatally. Mice were killed between postnatal days 7 and 26, and the pancreas was examined histologically. Apoptotic cells were visualized by the terminal deoxynucleotidyltransferase-mediated deoxy-UTP nick end labeling method, and proliferating cells were examined by immunohistochemistry for proliferating cell nuclear antigen. In nontransgenic mice, serum IGF-II was absent by 26 days, but mean (+/-SEM) values were 45+/-9 ng/ml (n = 5) in transgenic animals. A 2- to 3-fold rise in islet cell apoptosis was seen in normal animals between days 11 and 16, but this was substantially decreased in IGF-II transgenic mice (day 11; control, 12+/-1%; transgenic, 6+/-1%; P < 0.01; n = 5). Consequently, islets from IGF-II transgenic mice had a significantly greater mean area from days 11-16, but the proportions of beta- and alpha-cells and circulating insulin levels were not changed. Islet cell DNA synthesis was increased in transgenic mice on days 13 and 16. The total islet number per section did not alter. The results show that a persistent presence of circulating IGF-II postnatally alters endocrine pancreatic ontogeny in the mouse and largely prevents the wave of developmental apoptosis that precipitates beta-cell turnover in neonatal life.
在大鼠中,一部分胰腺β细胞在出生后第二周通过凋亡被清除,并由胰腺导管上皮的内分泌细胞新生所取代。这与胰腺胰岛素样生长因子II(IGF-II)表达的降低相吻合,并且IGF-II在体外已被证明可作为β细胞存活因子。为了研究IGF-II在体内是否调节β细胞凋亡,使用了一种IGF-II转基因小鼠模型,其中小鼠IGF-II在角蛋白启动子的驱动下在皮肤、肠道和子宫中过度表达,从而使循环中的IGF-II在出生后得以保留。在出生后第7至26天之间处死小鼠,并对胰腺进行组织学检查。通过末端脱氧核苷酸转移酶介导的脱氧UTP缺口末端标记法观察凋亡细胞,通过免疫组织化学检测增殖细胞核抗原检查增殖细胞。在非转基因小鼠中,到26天时血清IGF-II消失,但转基因动物的平均(±SEM)值为45±9 ng/ml(n = 5)。在正常动物中,11至16天之间胰岛细胞凋亡增加了2至3倍,但在IGF-II转基因小鼠中这一现象明显减少(第11天;对照组,12±1%;转基因组,6±1%;P < 0.01;n = 5)。因此,在11至16天期间,IGF-II转基因小鼠的胰岛平均面积明显更大,但β细胞和α细胞的比例以及循环胰岛素水平没有变化。在第13天和16天,转基因小鼠的胰岛细胞DNA合成增加。每切片的胰岛总数没有改变。结果表明,出生后循环中持续存在的IGF-II会改变小鼠内分泌胰腺的个体发生,并在很大程度上防止了引发新生期β细胞更新的发育性凋亡浪潮。
