吡格列酮对游离脂肪酸作用下βTC-3细胞GPR40表达的干预作用

目的探讨游离脂肪酸(FFA)作用下胰岛βTC-3细胞G蛋白受体40(GPR40)mRNA表达的改变以及吡格列酮(Piog)对此改变的干预作用。方法以βTC-3细胞为研究对象,分为对照组及FFA组(0.25,0.5及1mmol/L)。半定量RT-PCR方法检测GPR40的表达。用不同浓度的Piog(0,0.1,1,10μmol/L)预孵育βTC-3细胞6h,加入1mmol/LFFA继续孵育24h,半定量RT-PCR方法检测GPR40的表达。结果(1)FFA孵育12h后,各组间GPR40的表达差别无统计学意义。(2)FFA孵育24h后,与对照组比较,0.25mmol/LFFA组GPR40的表达无差异,但0.5mmol/L和1mmol/LFFA组GPR40表达下调(P<0.05);0.5mmol/L与1mmol/LFFA组比较GPR40表达差别无统计学意义。(3)与1mmol/LFFA组比较,0.1μmol/LPiog+1mmol/LFFA组GPR40mRNA表达无差异,而1μmol/LPiog+1mmol/LFFA组和10μmol/L+1mmol/LFFA组GPR40表达升高(P<0.01)。结论长期高浓度FFA作用能够下调βTC-3细胞GPR40的表达,而Piog有助于保护或减轻FFA水平异常导致的βTC-3细胞GPR40表达的损害。

The dimerization of ⊿~9-tetrahydrocannabinolic acid A(THCA-A)

The renewed interest in dimeric salicylates as broad-spectrum anti-inflammatory and antidiabetic agents provided a rationale to investigate the dimerization of the substituted salicylate D9-tetrahydrocannabinolic acid(THCA-A, 3 a) as a strategy to solve its instability to decarboxylation and to generate analogues and/or pro-drugs of this native pre-cannabinoid. Activation of the carboxylic group with the DCC-HOBt-DMAP protocol afforded a high yield of the OBt ester 4, that was next converted into the highly crystalline di-depsidic dimer 5 upon treatment with DMAP. The mono-depsidic dimer 6 was also formed when the reaction was carried out with partially decarboxylated THCA-A samples. The structure of the depsidic dimers was established by spectroscopic methods and by aminolysis of 5 into the pre-cannabinoid amide 7. Both dimers showed excellent shelf stability and did not generate significant amounts of D9-THC upon heating. However, only the didepsidic dimer 5 activated PPAR-g, the major target of pre-cannabinoids, but strong binding to serum proteins abolished this activity, also shielding it from the action of esterases.