Nkx6.2 synergizes with Cdx-2 in stimulating proglucagon gene expression

AIM: To investigate whether the transactivator of the proglucagon gene (Gcg), Cdx-2, synergizes with other transcription factors in stimulating Gcg expression and the trans-differentiation of Gcg-expressing cells. METHODS: We conducted affinity chromatography to identify proteins that interact with Cdx-2, using GST-tagged Cdx-2 against cell lysates from pancreatic InR1-G9 and intestinal GLUTag cell lines. This was followed by a mass-spectrometry analysis. From a potential Cdx-2 interaction protein identified, we examined its expression in pancreatic and gut endocrine cells, confirmed its interaction with Cdx-2 by GST-pull down and determined its effect in provoking Gcg expression in cell lines that do not express endogenous Gcg.RESULTS: We identified 18 potential Cdx-2 interacting proteins. One of them is Nkx6.2. This homeodomain (HD) protein is expressed in pancreatic α and intestinal endocrine L cells but not in insulin producing cell lines, inclu ding In111. Nkx6.2, but not Nkx6.1, was shown to intera ct with Cdx-2, detected by GST-pull down. Furthermore, Nkx6.2 was found to synergize with Cdx-2 in provoking Gcg expression when they were ectopically expressed in the In111 cell line. Finally, when Cdx-2 and Nkx6.2 were co-transfected into the undifferentiated rat intestinal IEC-6 cell line, it produced detectable amount of Gcg mRNA. CONCLUSION: Cdx-2 recruits Nkx6.2 in exerting its ef fect in stimulating Gcg expression. Our observations fur ther support the notion that multiple HD proteins, including Cdx-2 and Nkx6.2, are involved in the regulation of Gcg expression and the genesis of Gcg-producing cells.

清化颗粒对db/db小鼠胰高血糖素样肽-1合成和分泌的影响

目的:探讨清化颗粒对db/db小鼠肠道胰高血糖素样肽-1(GLP-1)合成和分泌的影响。方法:选取db/m小鼠为空白对照组,db/db糖尿病小鼠随机分为模型对照组和清化颗粒(低、中、高剂量)组,干预4周,观察小鼠糖代谢变化;ELISA法分析小鼠血清GLP-1的水平;qRT-PCR法检测小鼠回肠胰高血糖素原和激素原转化酶1/3(PC1/3)的mRNA水平;Western blot法检测小鼠回肠PC1/3的蛋白表达水平;组织病理学观察小鼠回肠组织形态变化。结果:与模型对照组比较,清化颗粒降低db/db糖尿病小鼠的空腹血糖(FBG)(P<0.01);提高血清GLP-1的浓度(P<0.01);上调小鼠回肠组织胰高血糖素原和PC1/3酶的mRNA水平(P<0.01);上调小鼠回肠组织PC1/3的蛋白表达水平(P<0.01);并具有剂量依赖效应。另外,清化颗粒明显改善db/db糖尿病小鼠回肠组织形态。结论:清化颗粒能够降低db/db糖尿病小鼠的血糖水平,提高血清GLP-1水平,上调胰高血糖素原和PC1/3的mRNA水平,促进肠道GLP-1的合成和分泌,改善回肠组织形态。

人源性高血糖素原基因的克隆

目的克隆人高血糖素原基因(proglucagonc DNA,PG cDNA),构建其真核表达质粒载体。方法从人切除脑组织中提取总RNA,并分离mRNA,经过逆转录-聚合酶链反应(RT-PCR)扩增出PGcDNA,并将其插入经BamHⅠ和EcoRⅠ双酶切的真核表达质粒载体pVITRO3中,构建重组质粒载体pVITRO3-PGcDNA。结果经过限制性酶切鉴定和测序证明,PGcD-NA全长543bp,编码181个氨基酸,并已插入到pVITRO3中。结论成功获得了PGcDNA,构建了含PGcDNA的真核表达质粒载体,为研究重组PG的功能奠定了基础。

十二指肠空肠旁路术对2型糖尿病GK大鼠肠道胰高血糖素原表达的影响

目的观察十二指肠空肠旁路术（duodenal-jejunal bypass，DJB）对2型糖尿病GK大鼠的降糖作用及对肠道胰高血糖素原（proglucagon，PG）表达的影响。方法雄性GK和Wistar大鼠各18只，GK大鼠随机分为手术组（A组）假手术组（B组），Wistar大鼠随机分为手术组（C组）和假手术组（D组），每组9只。检测术前及术后各组空腹血糖、血清GLP-1水平，同时口服葡萄糖耐量试验，并计算血糖曲线下面积；术后8周取各组大鼠肠道组织标本，采用RT—PCR检测术后肠道PGmRNA表达水平。结果术后第8周，A组空腹血糖由术前的（8．73±1．30）mmol／L下降到（5．86±0．57）mmol／L，差异有统计学意义（P〈0．05）；血糖曲线下面积由术前（60．23±5．14）mmol·k／L下降到（47．80±1．79）mmol·h／L，差异有统计学意义（P〈0．05）；空腹GLP-1由术前（7．69±0．74）pmol／L上升到（29．00±4．85）pmol／L，餐后GLP-1由术前（15．74±5．71）pmol／L上升到（45．78±7．26）pmol／L，差异有统计学意义（P均〈0．05）；A组术后回肠PGmRNA水平明显高于B组，差异有统计学意义（P〈0．05）。结论DJB能显著改善2型糖尿病大鼠的糖代谢，而对正常大鼠糖代谢无影响，手术的降糖作用可能与肠道胰高血糖素原表达增加有关。

黄芪多糖对高糖高脂饮食模型大鼠肠道甜味受体通路的影响

目的:探讨黄芪多糖对高糖高脂饮食模型大鼠肠道甜味受体味觉受体第一家族成员2(T1R2)/味觉受体第一家族成员3(T1R3)通路的影响。方法:SD大鼠随机分为正常组、高糖高脂组和黄芪多糖组。高糖高脂饲料组和黄芪多糖组大鼠给予高糖高脂饲料喂养16周,期间黄芪多糖组大鼠每日给予0. 7 g·kg^(-1)的APS灌胃8周。采集大鼠血清测定空腹血糖,总胆固醇(TC),甘油三酯(TG),高密度脂蛋白胆固醇(HDL-C)和低密度脂蛋白胆固醇(LDL-C)含量;采集大鼠肠道组织,采用实时荧光定量聚合酶链式反应(Real-time PCR)检测甜味受体通路T1R2,T1R3,α-味导素(Gαgust)和顺时受体电位阳离子通道5(TRPM5)以及胰高血糖素原(PG) mRNA的表达水平;蛋白免疫印迹法(Western blot)检测T1R2,Gαgust和胰高血糖素样肽(GLP-1)蛋白表达水平。结果:与正常组比较,高糖高脂组大鼠血清TC,TG和LDL-C含量明显升高,HDL-C含量明显降低(P <0. 05);肠道甜味受体通路中的T1R2,Gαgust和PG mRNA表达水平明显降低(P <0. 05);与高糖高脂组比较,黄芪多糖组大鼠血清TC,TG,LDL-C含量明显降低,HDL-C含量明显升高(P <0. 05),肠道甜味受体通路分子T1R2,T1R3,Gαgust,TRPM5以及PG mRNA表达水平明显升高(P <0. 05),T1R2,Gαgust和GLP-1蛋白表达明显升高;与模型组比较,黄芪多糖组T1R3 mRNA表达及T1R2,Gαgust,GLP-1蛋白表达水平均明显降低(P <0. 05)。结论:黄芪多糖可改善高糖高脂饮食模型大鼠脂代谢紊乱和肠道甜味受体通路的损伤。