维生素C通过调控脂肪形成相关基因的转录促进猪前体脂肪细胞的增殖与分化

探讨维生素C（Vit C）诱导猪前体脂肪细胞增殖分化最佳浓度及在分化过程中,5种脂肪形成相关基因peroxisome proliferator activated receptor gamma(PPARγ)和retinoid X receptor alpha(RXRα),脂肪细胞分化标志基因lipoprotein lipase (LPL),生脂基因phosphoenolpyruvate carboxykinase(PEPCK)、stearoyl CoA desaturase(SCD) mRNA表达时序性的变化. 以3　d龄猪前体脂肪细胞为实验对象,用Vit C诱导猪前体脂肪细胞增殖分化,分别在增殖分化第2、4、6和8 d收获细胞,利用MTT测定其增殖程度;油红O染色提取法检测其脂肪含量;采用SQ RT PCR法检测脂肪生成相关基因PPARγ、RXRα、LPL、PEPCK和SCD mRNA表达的变化. 结果显示,PPARγ mRNA在诱导分化第2 d时有低水平表达,在诱导分化过程中表达量逐步升高,在终末分化阶段仍保持高水平表达;RXRα mRNA在诱导分化第2和4 d表达量很低,诱导分化第6 d时表达增加.在诱导分化第8 d,RXRα mRNA表达与第6 d相比差异不显著,直至终末分化. 脂肪细胞分化标志基因LPL在第2 d开始表达,第4和6 d逐步升高,在终末分化阶段仍保持高水平的表达;生脂基因PEPCK和SCD mRNA在第2和4 d开始表达,第6和8 d仍保持高水平的表达. 研究结果表明,100 μmol/L的Vit C促进猪前体脂肪细胞增殖能力最强;250 μmol/L Vit C能显著促进猪前体脂肪细胞分化. 其作用机制可能是通过对转录因子PPARγ和RXRα及标志基因LPL mRNA时序性表达的调控来进行的,促进生脂基因的表达,从而诱导脂肪细胞的分化.     

视黄酸X受体α促进猪前体脂肪细胞分化

采用细胞转染、油红O染色、油红O染色提取法、GPDH活性测定、semi-qRT-PCR等方法研究了视黄酸X受体α (retinoic acid X receptor α, RXRα)在猪原代前体脂肪细胞分化中的作用及其机理.结果表明,转染pRXRα-EGFP促进了猪前体脂肪细胞RXRα 的表达,脂肪细胞分化能力随之增强, 脂肪细胞GPDH活性、分化转录因子PPARγ和C/EBPαmRNA表达水平均显著升高(P<0.05). 结果提示,RXRα可能通过调控过氧化物酶体增殖物激活受体γ(peroxisome proliferators-activated receptor-γ, PPARγ)和CAAT/增强子结合蛋白家族（CCAAT/enhancer binding proteins, C/EBP）C/EBPα 基因表达变化促进猪前体脂肪细胞分化.     

过表达miR-103促进猪前体脂肪细胞分化

为阐明miR-103在猪前体脂肪细胞分化过程中的调控作用,采用Real-time PCR检测猪前体脂肪细胞成脂分化过程中的miR-103表达谱,明确了其在分化过程中的表达趋势;使用miR-103的腺病毒超表达载体感染猪原代脂肪细胞,随后采用Real-time PCR和Western blotting分别检测成脂标记基因PPARγ、aP2的mRNA和蛋白表达量变化;油红O染色观察腺病毒miR-103侵染的前体脂肪细胞诱导分化第8天的成脂情况。结果显示,miR-103的表达量随着脂肪细胞分化而增加,在miR-103超表达的猪原代脂肪细胞的诱导分化过程中,成脂标记基因PPARγ、aP2的表达量与对照相比显著升高,分化第8天观察到明显的脂滴。说明miR-103能够促进猪前体脂肪细胞分化。     

黄芩素对猪前体脂肪细胞增殖分化的影响

研究黄芩素(BAI)对猪前体脂肪细胞增殖分化的影响,并探讨其可能的作用机制。原代培养猪前体脂肪细胞,采用油红O染色观察细胞分化的形态学变化;MTT检测细胞增殖状况;油红O染色提取定量分析细胞内脂肪生成及细胞分化程度;分光光度法测定脂肪酸合酶(FAS)的活性;逆转录-聚合酶链反应(RT-PCR)检测分化特异基因过氧化物酶体增殖物激活受体γ2(PPARγ2)mRNA表达变化。结果显示,前体脂肪细胞在分化成脂肪细胞的过程中,其形态由梭形变成椭圆形、圆形,细胞内充满大小不一的脂滴;BAI浓度在160～640μmol/L时显著抑制其增殖(P<0.05)、BAI浓度为40～320μmol/L时显著抑制PPARγ2mRNA表达和FAS的活性,并抑制细胞分化(P<0.05)。以上结果说明,BAI对前体脂肪细胞增殖分化均有一定抑制作用,BAI可能通过抑制PPARγ2mRNA表达和降低FAS活性,从而抑制猪前体脂肪细胞分化。     

Txnip基因siRNA慢病毒表达质粒构建及促进猪前体脂肪细胞分化

硫氧还蛋白互作蛋白(thioredoxin interacting protein, Txnip)是一种氧化还原调节蛋白质,与硫氧还蛋白结合并抑制其活性,调节细胞氧化还原状态,影响细胞多种生理过程,然而其在猪脂肪细胞分化中的作用尚不明确。本文设计合成3对靶向猪Txnip基因的shRNA寡核苷酸,分别连接于重组慢病毒载体pGLV_3/H_1/GFP+Puro构建siRNA表达质粒。测序验证后,与包装质粒共转染293T细胞,获得滴度1×10~8 pfu/mL的慢病毒干扰质粒。以MOI值100转染原代培养猪前体脂肪细胞,转染率均达80%以上,其中Txnip-shRNA-2转染细胞Txnip基因沉默率达75%。转染Txnip-shRNA-2的猪前体脂肪细胞用成脂分化培养液诱导后,每隔1 d检测细胞成脂分化及相关基因表达。结果发现,其分化比阴性对照质粒转染或未转染细胞显著增强(P<0.05),PPARγ和FAS mRNA表达水平显著提高(P<0.05)。本文构建siRNA慢病毒表达质粒能有效干扰猪Txnip基因表达,Txnip表达沉默可通过上调PPARγ表达促进猪前体脂肪细胞分化。本研究提示,Txnip可能是猪脂肪细胞分化的抑制因子。     

9-顺式维甲酸在原代培养猪前体脂肪细胞分化中的调控作用

采用RT-PCR、油红O染色法、油红O染色提取法和分光光度计法,探讨不同浓度9-顺式维甲酸(9-cisRA)(0-10$mol/L)对体外原代培养猪前体脂肪细胞分化的影响及其可能机制。结果表明,9-cisRA在脂肪细胞分化中因浓度不同而发挥不同作用。低浓度9-cisRA(0-10nmol/L)促进前体脂肪细胞分化,并上调RXRα、PPARγmRNA表达,增加前体脂肪细胞分化标志酶3-磷酸甘油脱氢酶(glyc-erol-3-phosphate dehydrogenase,GPDH)的活性;高浓度9-cisRA(100nmol/L-10$mol/L)则抑制前体脂肪细胞分化,并下调RXRα、PPARγmRNA表达,减少GPDH的活性。结果提示9-cisRA在猪前体脂肪细胞分化中,可能通过调控RXRα和PPARγ基因表达变化来发挥其促进或抑制作用。     

Leptin过表达对猪前脂肪细胞脂滴形成的研究

研究Leptin过表达对猪前脂肪细胞脂滴形成的影响,旨为进一步研究Leptin与脂质代谢相关的分子机制奠定理论基础。选取Leptin过表达与野生型猪皮下脂肪组织,在无菌条件下分离前脂肪细胞进行传代培养并诱导分化形成脂滴,通过油红O和Bodipy染色后观察脂滴面积并分析脂质的含量,利用Q-PCR检测脂滴形成相关基因mRNA的表达水平。诱导4 d后可分化形成脂滴,油红O和Bodipy染色的结果显示,Leptin过表达猪前脂肪细胞脂滴数量和甘油三酯含量显著低于野生型(P0.05);且脂质合成相关基因PPARγ、SCAP、SREPB1和PLIN2的表达水平显著低于野生型(P0.01)。结果表明,过表达Leptin可促使猪前脂肪细胞中PPARγ、SREPB1、SCAP、PLIN2基因的表达下调,进而抑制脂滴形成。     

Lnc-RAP3对小鼠3T3-L1前脂肪细胞分化的影响

长链非编码RNA(long non-coding RNA,lnc RNA)是一类长度大于200nt、没有长开放阅读框架但往往具有m RNA结构特征的RNA,可以在转录及转录后水平参与基因的表达调控。近年来,有研究证实lnc RNA对脂肪生成具有重要作用。Lnc-RAP3位于小鼠(Mus musculus)17号染色体,其表达量在小鼠脂肪细胞分化前后呈现显著差异,但其具体的生物学功能尚不清楚。为探讨lnc-RAP3在小鼠3T3-L1前脂肪细胞成脂分化中的作用,本文首先构建了lnc-RAP3的真核表达载体pc DNA3.1-RAP3,利用脂质体将pc DNA3.1-RAP3和人工合成的lnc-RAP3的si RNAs分别转染3T3-L1前脂肪细胞,并对转染后的细胞进行诱导分化,并通过油红O染色、q RT-PCR检测成脂分化相关基因表达等方法比较过表达和敲降lnc-RAP3对3T3-L1前脂肪细胞成脂分化的影响。结果显示,过表达lnc-RAP3后,细胞内脂滴聚集显著减少(P0.05),在诱导分化第0 d、2 d和4 d时C/EBPα、Glut4、PPARγ、LPL和FAS的表达水平均呈显著(P0.05)或极显著(P0.01)下降;敲降lnc-RAP3后,细胞内脂滴聚集显著增多(P0.05),同时在诱导分化第0 d、2 d时PPARγ、LPL、C/EBPα、FAS和Glut4的表达水平呈显著(P0.05)或极显著(P0.01)升高。本研究结果表明,lnc-RAP3可能通过影响成脂分化相关基因的表达来抑制3T3-L1前脂肪细胞的成脂分化。     

猪前体脂肪细胞的分离培养

在比较组织块法和消化法分离培养猪前体脂肪细胞的基础上,通过对前体脂肪细胞增殖与分化过程中细胞的形态学变化、生长曲线、油红O染色以及脂肪细胞特异性标志基因脂蛋白脂酶（lipoprotein lipase,LPL）和过氧化物体增殖剂活化受体γ（peroxisome proliferators-activated receptor γ,PPARγ）表达的研究,证明用消化法可从猪的脂肪组织中分离获得大量的前体脂肪细胞,其生长旺盛,可见自发充脂;传代细胞经诱导培养后,充脂率大幅度提高,脂肪特异性标志基因表达增强。这为深入研究脂肪细胞增殖与分化以及猪体脂肪沉积提供了一个较好的模型。     

miR-130a在猪皮下脂肪细胞分化中的调节作用

为研究miR-130a对猪皮下脂肪细胞分化的影响及可能机制,本试验分离猪皮下脂肪前体细胞,诱导分化为成熟脂肪细胞,检测脂肪细胞分化过程中脂滴变化及miR-130a及其可能靶基因TNF-α和PPARγ的表达模式.同时合成miR-130a mimics及inhibitor对细胞进行转染,并以乱序序列作为阴性对照(NC).细胞转染24 h后进行诱导分化,连续诱导8 d,检测各处理细胞的聚脂情况及甘油三酯含量变化,荧光定量PCR检测脂肪细胞分化相关基因的表达变化.结果显示,猪皮下脂肪前体细胞分化过程中脂滴逐渐变大增多,miR-130a、TNF-α和PPARγ的表达模式具有一定的相似性.转染结果显示,相对于对照组,miR-130a mimics转染组细胞脂滴减少变小,甘油三酯含量降低(P0.05),脂肪细胞分化相关基因LPL、PPARγ、adiponectin、FASN和葡萄糖转运相关基因GLUT1,GLUT4以及JNK通路上的PDE3B的表达均比对照组显著下调(P0.01);而miR-130a inhibitor转染组细胞则脂滴增多,甘油三酯含量提高(P0.05),但大部分分化相关基因的表达与对照组无显著差异,提示miR-130a可能不只通过单一的靶基因影响脂肪细胞分化.其结果为后续深入研究miR-130a调节猪脂肪细胞分化的通路及机制奠定基础.     

Knockdown of KLF9 promotes the differentiation of both intramuscular and subcutaneous preadipocytes in goat

ABSTRACT

KLF9 is reported to promote adipocyte differentiation in 3T3-L1 cells and pigs. However, the roles of KLF9 in adipocytes differentiation of goat remain unknown. In this study, the expression profiles of KLF9 were different between subcutaneous and intramuscular preadipocytes of goat during differentiation process. After silencing KLF9 gene, the lipid droplets were increased in both two types of adipocytes. In subcutaneous preadipocyte with silencing KLF9, the expressions of C/EBPβ, PPARγ, LPL, KLF1-2, KLF5, and KLF17 genes were up-regulated, while KLF12, KLF4, and KLF13 genes were down-regulated in expression level. In intramuscular preadipocyte, aP2, C/EBPα, KLF2-3, KLF5, and KLF7 gene were up-regulated, and Pref-1 gene was down-regulated. In addition, the binding sites of KLF9 existed in the promoters of aP2, C/EBPα, C/EBPβ, LPL and Pref-1. Taken together, KLF9 play a negative role in the differentiation of both intramuscular and subcutaneous preadipocytes in goats, but the functional mechanism may be different.     

Isomers of conjugated linoleic acid modulate human preadipocyte differentiation

Conjugated linoleic acids (CLAs) reduce fat deposition in several mammalian species. Among the proposed mechanisms for this effect are reduced preadipocyte proliferation and differentiation. We measured proliferation and differentiation of cultured human preadipocytes treated with CLAs. Preadipocytes were differentiated with insulin, hydrocortisone, transferrin, and 10% fetal bovine serum, with isobutyl-methylxanthine included for the first 2 d. The differentiation medium contained 200 microM oleic acid (C18:1), 50 microM cis-9,trans-11-CLA (9,11-CLA), or 50 microM trans-10,cis-12-CLA (10,12-CLA); the negative control medium contained no added fatty acid, and the cells did not differentiate. Cell number increased three to four times during the 17 d of differentiation, but was 30-35% lower in the CLA-treated cells than in the negative control cells. Compared with the negative control cells, differentiation was increased in the cells treated with C18:1 (increased Oil Red O-stained material [OROSM], triacylglycerol, glycerol 3-phosphate dehydrogenase activity [GPDH], peroxisome proliferator-activated receptor-gamma [PPAR gamma] messenger ribonucleic acid [mRNA], and lipoprotein lipase [LPL] mRNA). In effect, the C18:1-treated cells act as a positive control to demonstrate the differentiation capacity of each cell lot. Both 9,11-CLA- and 10,12-CLA-treated cells had increased differentiation (increased OROSM, triacylglycerol, GPDH, PPAR gamma, and LPL) compared with the negative control cells. The data suggest that early in differentiation when de novo fatty acid (FA) synthesis is limited and competition for FAs by membrane and triacylglycerol synthetic pathways is great, human preadipocytes do not differentiate unless a PPAR gamma ligand is added. Either CLA isomer or C18:1 can provide such a ligand.     

The adipokine Chemerin induces lipolysis and adipogenesis in bovine intramuscular adipocytes

The adipokine Chemerin is reported to regulate adipogenesis and glucose homeostasis in vivo and in 3T3-L1 cells. Our team is focused on the role of Chemerin in metabolism and intramuscular adipocyte differentiation because intramuscular fat is the basic material for the formation of marbling in livestock and poultry meat. In this study, bovine intramuscular mature adipocytes were cultured in medium with Chemerin, and the process of lipolysis of mature adipocytes and the adipogenesis of de-differentiated preadipocytes were investigated. The results showed that Chemerin induced significant lipolytic metabolism in intramuscular mature adipocytes, indicated by increased levels of glycerol, FFA, and up-regulated expression of the lipolysis critical factors HSL, LPL, and leptin. Meanwhile, the expressions of adipogenic key factors PPARγ, C/EBPα, and A-FABP were decreased by Chemerin during lipolysis or dedifferentiation in mature adipocytes. The de-differentiated preadipocytes could re-differentiate into mature adipocytes. Intriguingly, the formation of cells’ lipid droplets was promoted by Chemerin during preadipocyte differentiation. In addition, mRNA and protein expressions of PPARγ, C/EBPα, and A-FABP were up-regulated by Chemerin during preadipocytes differentiation. These results suggest that Chemerin promotes lipolysis in mature adipocytes and induces adipogenesis during preadipocyte re-differentiation, further indicating a dual role for Chemerin in the deposition of intramuscular fat in ruminant animals.

     

Dehydroabietic acid activates peroxisome proliferator-activated receptor-γ and stimulates insulin-dependent glucose uptake into 3T3-L1 adipocytes

Dehydroabietic acid (DAA) is a food-derived terpenoid with various bioactivities. Our previous study has revealed that DAA activates peroxisome proliferator-activated receptor-γ (PPARγ) in luciferase assay and suppresses chronic inflammation in obese adipose tissues. In this study, we examined the effects of DAA on adipocyte differentiation. DAA treatment stimulated the adipocyte differentiation of 3T3-L1 preadipocytes. The DAA treatment increased the mRNA expression levels of adipocyte differentiation marker genes such as aP2, lipoprotein lipase (LPL), and PPARγ. In particular, the expression level of adiponectin, which is an adipocytokine with stimulatory effects on insulin sensitivity, was increased at both the mRNA and protein levels by the DAA treatment. Moreover, the DAA treatment stimulated insulin-dependent glucose uptake into differentiated 3T3-L1 adipocytes. These findings indicate that DAA stimulates adipocyte differentiation and insulin sensitivity in 3T3-L1 cells, suggesting that DAA is a valuable food-derived compound for the management of metabolic syndrome.     

罗格列酮对猪脂肪前体细胞分化过程中聚脂相关基因表达模式的影响

为了解罗格列酮对猪脂肪前体细胞诱导分化过程的影响, 利用胶原酶消化法分离猪皮下脂肪前体细胞, 采用含50 nmol/L胰岛素、100 nmol/L地塞米松及0.25 mmol/L 3-异丁基-1-甲基黄嘌呤的分化培养液Ⅰ(对照组)和在分化培养液Ⅰ中添加100 nmol/L罗格列酮的分化培养液Ⅱ(实验组)两种诱导分化方法对脂肪前体细胞进行诱导分化, 借助实时定量RT-PCR方法检测了细胞分化过程中聚脂相关基因的表达。结果显示: 罗格列酮对PPARγ、C/EBPα、FABP4、FASN和GPAT基因的表达有显著的上调作用, 而对PPARα有一定的下调作用。试验组中PPARα、PPARγ、C/EBPα、FABP4、FASN和GPAT等基因分别于48 h、48 h、48 h、108 h、60 h和24 h达到表达高峰, 此时的表达量分别是诱导前的1.7、48、3.3、487.5、5.8和3.6倍, GPAT同PPARα和FASN基因表达量间均达到显著相关(P<0.05); 而对照组中PPARα、PPARγ、C/EBPα、FABP4、FASN和GPAT等基因分别于84 h、96 h、48 h、96 h、36 h和36 h达到表达高峰, 此时的表达量分别是诱导前的2.1、11、1.6、216.5、3.5和2.8倍, GPAT同PPARα和FASN基因表达量间均达到极显著相关(P<0.01)。本实验结果表明: 罗格列酮不仅可以极大的促进PPARγ和C/EBPα基因的表达, 还能让其协同达到表达高峰; PPARγ和C/EBPα可能是调控猪脂肪前体细胞分化的关键转录因子; 在脂肪形成过程中, 甘油脂类的生物合成可能发生较早, 同时PPARα可能主要参与甘油脂类生物合成的调控。     

ABCA1和PPARγ与糖尿病动脉粥样硬化关系的研究

目的：研究ATP结合盒转运体A1（ABCA1）在多种糖尿病特有因素刺激下在巨噬细胞中的表达,以及PPARγ激动剂干预后其表达的变化,探讨ABCA1及PPARγ在糖尿病大血管并发症发展中的作用机制。从而为研究糖尿病大血管并发症的发生机制及防治提供一定的理论依据。方法：以巨噬细胞为研究对象,体外模拟糖尿病状态,分别以高葡萄糖、高胰岛素和糖基化终末产物刺激巨噬细胞,检测细胞中ABCA1表达的变化;以PPARγ激动剂预处理巨噬细胞后,再以上述因素刺激细胞,分别检测巨噬细胞中ABCA1的表达并比较。结果：高葡萄糖、高胰岛素和糖基化终末产物（AGE）可作为独立因素,导致细胞中ABCA1表达减少（P〈0.05）。PPARγ激动剂预处理后,ABCA1表达量增加（P〈0.05）。结论：糖尿病状态下,一些糖尿病特有的刺激因素如：高葡萄糖、高胰岛素和糖基化终末产物等作为独立因素使ABCA1表达减少,可能是糖尿病患者动脉粥样硬化发生率较非糖尿病人群增高的原因。PPARγ激动剂干预后,糖尿病状态下ABCA1的表达增加,这提示我们应用PPARγ激动剂可能延缓糖尿病患者动脉硬化进展。     

Inhibition of preadipocyte differentiation by myostatin treatment in 3T3-L1 cultures

Myostatin, a new TGF-beta family member, is known as a muscle growth inhibitor, but its role in adipocyte development has not been studied. To test the role of Myostatin in 3T3-L1 preadipocyte differentiation, we treated cultured 3T3-L1 preadipocytes with Myostatin dissolved in 0.1% trifluoroacetic acid (TFA) during differentiation after they had become confluent. Myostatin treatment significantly decreased glycerol-3-phosphate dehydrogenase (GPDH) activity and oil Red-O staining compared to controls that did not receive Myostatin. Western blot analysis showed that the expression levels of CCAAT/enhancer binding protein alpha (C/EBP alpha) and peroxisome proliferator-activated receptor gamma (PPAR gamma) were significantly decreased by Myostatin treatment (P < 0.05). However, the expression of C/EBP beta was not significantly changed by the treatment (P > 0.05). From RT-PCR result, the relative level of leptin mRNA in Myostatin-treated cells was not significantly different (P > 0.1) from the level in cells without Myostatin treatment. Our data show that Myostatin, a secreted protein from muscle, inhibits preadipocyte differentiation in 3T3-L1 cells, which is mediated, in part, by altered regulation of C/EBP alpha and PPAR gamma.