联合检测CHI3L1、AFP和GGT在乙肝相关肝癌患者中的相关性研究

目的探讨血清壳多糖酶3样蛋白1(chitinase-3-like protein 1,CHI3L1)、甲胎蛋白(alpha fetoprotein,AFP)和γ-谷氨酰转移酶(γ-glutamyl transferase,GGT)检测在乙型肝炎病毒(hepatitis B virus,HBV)感染相关肝癌诊断中的临床应用价值。方法选取2021年7月—2023年7月在玉林市第一人民医院就诊HBV病毒感染相关的50例肝癌患者,50例肝硬化患者,50例慢性乙型肝炎患者以及50名同期健康体检者作为研究对象。比较4组研究对象血清中CHI3L1、AFP、GGT、丙氨酸氨基转移酶(alanine aminotransferase,ALT)、天门冬氨酸氨基转移酶(aspartate aminotransferase,AST)等水平的差异,用受试者工作特征(receiver operating characteristic curve,ROC)曲线评估各指标在肝癌中的诊断价值。结果肝炎组、肝硬化组、肝癌组的CHI3L1、AST、ALT水平均高于对照组,肝癌组AFP、GGT水平高于对照组,差异有统计学意义(P<0.05)。与肝炎组比较,肝硬化组及肝癌组的CHI3L1、AFP、GGT、AST、ALT水平均升高,差异有统计学意义(P<0.05)。与肝硬化组比较,肝癌组的CHI3L1、AFP、GGT、AST水平均升高,差异有统计学意义(P<0.05)。ROC曲线分析显示,CHI3L1、AFP、GGT联合时的曲线下面积(area under the curve,AUC)最大(AUC=0.936)。Spearman相关分析结果显示,CHI3L1与AST呈正相关(r=0.414,P=0.003),AFP与GGT呈正相关(r=0.437,P=0.002),AFP与AST呈正相关(r=0.504,P<0.001),GGT与AST呈正相关(r=0.759,P<0.001),GGT与ALT呈正相关(r=0.636,P<0.001)。结论CHI3L1、AFP及GGT联合检测可提高肝癌的诊断价值,对临床肝癌患者诊疗有重要作用。

Evaluation of trabecular meshwork-specific promoters in vitro and in vivo using scAAV2 vectors expressing C3 transferase

AIM:To evaluate the potential of two trabecular meshwork(TM)-specific promoters,Chitinase 3-like 1(Ch3L1)and matrix gla protein(MGP),for improving specificity and safety in glaucoma gene therapy based on self-complementary AAV2(scAAV2)vector technologies.METHODS:An scAAV2 vector with C3 transferase(C3)as the reporter gene(scAAV2-C3)was selected.The scAAV2-C3 vectors were driven by Ch3L1(scAAV2-Ch3L1-C3),MGP(scAAV2-MGP-C3),enhanced MGP(scAAV2-eMGP-C3)and cytomegalovirus(scAAV2-CMV-C3),respectively.The cultured primary human TM cells were treated with each vector at different multiplicities of infections.Changes in cell morphology were observed by phase contrast microscopy.Actin stress fibers and Rho GTPases/Rho-associated protein kinase pathway-related molecules were assessed by immunofluorescence staining,real-time quantitative polymerase chain reaction and Western blot.Each vector was injected intracamerally into the one eye of each rat at low and high doses respectively.In vivo green fluorescence was visualized by a Micron III Retinal Imaging Microscope.Intraocular pressure(IOP)was monitored using a rebound tonometer.Ocular responses were evaluated by slit-lamp microscopy.Ocular histopathology analysis was examined by hematoxylin and eosin staining.RESULTS:In TM cell culture studies,the vectormediated C3 expression induced morphologic changes,disruption of actin cytoskeleton and reduction of fibronectin expression in TM cells by inhibiting the Rho GTPases/Rhoassociated protein kinase signaling pathway.At the same dose,these changes were significant in TM cells treated with scAAV2-CMV-C3 or scAAV2-Ch3L1-C3,but not in cells treated with scAAV2-eMGP-C3 or scAAV2-MGP-C3.At lowinjected dose,the IOP was significantly decreased in the scAAV2-Ch3L1-C3-injected eyes but not in scAAV2-MGPC3-injected and scAAV2-eMGP-C3-injected eyes.At highinjected dose,significant IOP reduction was observed in the scAAV2-eMGP-C3-injected eyes but not in scAAV2-MGP-C3-injected eyes.Similar to scAAV2-CMV-C3,scAAV2-Ch3L1-C3 vector showed efficient transduction both in the TM and corneal endothelium.In anterior segment tissues of scAAV2-eMGP-C3-injected eyes,no obvious morphological changes were found except for the TM.Inflammation was absent.CONCLUSION:In scAAV2-transduced TM cells,the promoter-driven efficiency of Ch3L1 is close to that of cytomegalovirus,but obviously higher than that of MGP.In the anterior chamber of rat eye,the transgene expression pattern of scAAV2 vector is presumably affected by MGP promoter,but not by Ch3L1 promoter.These findings would provide a useful reference for improvement of specificity and safety in glaucoma gene therapy using scAAV2 vector.

DNMT1、β-catenin和P-GSK-3β在结肠癌组织中的表达

目的探讨DNA甲基转移酶1(DNMT1)、β-连环素(β-catenin)和磷酸化糖原合成酶激酶(P-GSK-3β)在结肠癌中的表达及其与肿瘤分化程度和淋巴结转移等的关系。方法采用荧光定量PCR检测62例原发性结肠癌患者癌组织及21例正常大肠黏膜组织中DNMT1、β-catenin和GSK的表达,采用Westernblot方法验证蛋白的表达情况。结果结肠癌组织中DNMT1、β-catenin和P-GSK-3β表达程度显著高于正常组织。DNMT1在低分化程度的癌组织间相对含量高,β-catenin在肿瘤的不同分化程度及有无淋巴结转移的癌组织间相对含量的差异有统计学意义,而P-GSK-3β的组间比较无显著性差异。结论DNMT1、β-catenin和P-GSK-3β的活性改变与结肠癌有一定的相关性。

应用半乳糖表型差异高效筛选α-1,3半乳糖苷转移酶基因缺失的猪成纤维细胞

【目的】筛选α-1,3半乳糖苷转移酶(α1,3galactosyl transferase,GGTA1)基因缺失的猪成纤维细胞。【方法】用同源重组载体pBS-GGTA1-SKO和pBS-GGTA1-DKO电转染GGTA1单等位基因敲除(GGTA1+/-)的五指山小型猪胎儿成纤维细胞,利用磁激活细胞分选(MACS)、MACS联合流式细胞术(FACS)、TcdA联合FACS等3种方法进行细胞筛选;对MACS筛选获得的单细胞克隆进行PCR和FACS鉴定,对MACS联合FACS、TcdA联合FACS获得的细胞集落进行PCR鉴定。【结果】经MACS筛选获得了11个细胞克隆,经鉴定2个是GGTA1-/-细胞克隆,阳性率为18.2%;MACS联合FACS筛选获得了3个细胞克隆,经鉴定无GGTA1-/-细胞克隆,阳性率为0;TcdA联合FACS筛选获得了3个细胞克隆,经鉴定均为GGTA1-/-细胞克隆,阳性率为100%。【结论】MACS法筛选和TcdA联合FACS法筛选这2种方法均可以高效筛选出GGTA1双等位基因缺失的猪成纤维细胞,可用于进一步制备供异种器官移植的基因修饰小型猪。

胃癌组织中BNIP3基因甲基化及其与DNMT1表达的关系

目的探讨人胃癌组织DNMT1表达及其与BNIP3基因甲基化状态的关系。方法收集120例手术切除并经病理学证实的胃癌组织及其相应的癌旁正常组织,采用甲基化特异性PCR（MSP）方法检测胃癌组织及其相应癌旁组织BNIP3基因甲基化状态,采用免疫组化SP法检测BNIP3基因及DNMT1基因的蛋白表达水平。结果 120例胃癌组织中有72例发生了BNIP3基因甲基化,甲基化阳性率为60.0%,其相应癌旁正常组织有5例发生了BNIP3甲基化,甲基化阳性率为4.2%,差异有统计学意义（χ~2=85.839,P〈0.01）,胃癌组织中BNIP3基因甲基化状态与患者性别、年龄、肿瘤大小、肿瘤分期无相关性（P〉0.05）,而与分化程度及淋巴结转移情况有相关性（P〈0.05）,胃癌组织中BNIP3蛋白的表达率为17.5%（21/120）,显著低于其癌旁正常组织（80.0%,96/120）,差异有统计学意义（χ~2=93.809,P〈0.01）,胃癌组织中DNMT1蛋白的表达率为75.0%（90/120）,显著高于其癌旁正常组织（5.8%,7/120）,差异有统计学意义（χ~2=119.195,P〈0.01）。胃癌组织中BNIP3蛋白与DNMT1蛋白的表达呈负相关（r=-0.542,P〈0.01）。结论 DNMT1高表达可能导致BNIP3蛋白表达减少,从而参与了胃癌的发生。

肝癌组织中SOCS1、GSTP1及DKK3基因甲基化状态及与临床病理的关系

目的分析肝癌组织中细胞因子信号转导抑制因子1(SOCS1)、谷胱甘肽S-转移酶P1(GSTP1)及Dickkopf相关蛋白3(DKK3)基因甲基化状态及与临床病理的关系。方法取2015年1月—2019年12月在本院接受手术治疗的肝癌患者的癌组织及癌旁组织各70例。另选取同期在本院接受肝胆外科手术术后病理证实为正常肝组织20例。比较肝癌组织、癌旁组织、正常肝组织SOCS1、GSTP1、DKK3基因甲基化状态及不同临床病理的肝癌组织SOCS1、GSTP1、DKK3基因甲基化状态,分析肝癌组织SOCS1、GSTP1、DKK3基因甲基化状态与临床病理的关系。结果正常肝组织未见SOCS1、GSTP1、DKK3基因甲基化现象;肝癌组织SOCS1、GSTP1、DKK3基因甲基化阳性率显著高于癌旁组织(P<0.01);乙型肝炎表面抗原(HBsAg)阳性肝癌患者SOCS1基因甲基化阳性率显著高于HBsAg阴性患者,有血管侵犯的肝癌组织GSTP1基因甲基化阳性率显著高于无血管侵犯的肝癌组织,有肝硬化的肝癌组织DKK3基因甲基化阳性率显著高于无肝硬化的肝癌组织(P<0.05,P<0.01);肝癌组织SOCS1基因甲基化与HBsAg呈正相关、GSTP1基因甲基化与血管侵犯呈正相关、DKK3基因甲基化与肝硬化呈正相关(P<0.05,P<0.01)。结论肝癌组织及癌旁组织均存在SOCS1、GSTP1、DKK3基因甲基化现象,且肝癌组织SOCS1、GSTP1、DKK3基因甲基化阳性率高于癌旁组织,并分别与HBsAg、血管侵犯、肝硬化密切相关。

Role of microRNA-21 in uveal melanoma cell invasion and metastasis by regulating p53 and its downstream protein

AIM： To reveal the insight mechanism of liver metastasis in uveal melanoma, we investigated cell functions of microRNA-21 in three different uveal melanoma cell lines and analyze the relationship of target gene p53 and its downstream targets which been found significant expression in our previous study.METHODS： Quantitative real-time polymerase chain reaction （qRT-PCR） was used to detect microRNA-21 expression in normal uveal tissue and uveal melanoma cell lines. Lenti-virus expression system was used to construct OCM-1, MuM-2B and M619 cell line with stable overexpression and inhibition of microRNA-21. In vitro cell function tests such as cell proliferation, cell apoptosis, cell circle and abilities of migration and invasion were examined by MTT, BrdU assay, flow cytometry, transwell assay and Matrigel invasion assay respectively. The target gene was predicted by bioinformatics and confirmed by using a dual luciferase reporter assay. The expression of p53 and its suspected downstream targets LIM and SH3 protein 1 （LASP1） and Glutathione S Transferase pi （GST-Pi） were determined by qRT-PCR in mRNA level and western blotting analysis in protein level. Finally, the effect of microRNA-21 in a xenograft tumor model was assessed in four-week-old BALB/c nude mice. RESULTS： Compared to normal uveal melanoma, expressions of microRNA-21 were significantly higher in uveal melanoma cell lines. Overexpression of microRNA-21 promoted proliferation, migration, and invasion of OCM-1, M619 and MuM-2B cells, while inhibition of microRNA-21 reveal opposite effects. Wild type p53 was identified as a target gene of microRNA-21-3p, and proved by dual luciferase reporter assay. Up-regulated microRNA-21 inhibited the expression of wild type p53 gene, and the increased expression of LASP1 in mRNA level and protein level, while down-regulated microRNA-21 presented opposite way. However, GST-pi showed the potential pattern as expected, but relative mRNA level showed no statistically significant difference in OCM-1 cells. Furthermore, the mRNA expression of GST-pi was decreased in microRNA-21 overexpressing MuM-2B, and increased in M619 cells with inhibition of microRNA-21. In vivo, inhibition of microRNA-21 reduced tumor growth with statistically significant difference.CONCLUSION： These findings provide novel insight into molecular etiology of microRNA-21 in uveal melanoma cell lines, and suggest that microRNA-21 might be a potential candidate for the diagnosis and prognostic factor of human uveal melanoma in future.

GAL3ST1对肝细胞癌肿瘤进展的影响及机制研究

目的探究半乳糖-3-O-磺酰基转移酶1(GAL3ST1)对肝细胞癌(HCC)进展的影响及机制。方法以高转移人肝癌细胞株(MHCC97H)为研究对象,分别转染MHCC97H-GAL3ST1 OE上调GAL3ST1表达(GAL3ST1 OE组)、MHCC97H-GAL3ST1 KD下调GAL3ST1表达(GAL3ST1 KD组),另设不作任何处理的Ctrl组。采用MTT法检测各组细胞的增殖情况;流式细胞术检测各组细胞周期和凋亡情况;Western blotting检测鞘脂代谢通路蛋白的表达;观察小鼠皮下移植瘤的生长情况;实时荧光定量PCR(qPCR)检测各组UGT8和GALC mRNA的表达。结果培养24、48和72 h后,GAL3ST1 OE组细胞存活率分别为(127.27±2.47)%、(152.45±2.41)%和(174.62±0.78)%,均高于Ctrl组的(100±0.0)%、(125.86±1.84)%和(148.17±1.94)%,差异有统计学意义(P<0.05)。GAL3ST1 OE组S期细胞比例为(14.95±0.95)%,低于Ctrl组的(30.27±0.24)%,差异有统计学意义(P<0.05)。GAL3ST1 OE组早期及晚期细胞凋亡率分别(0.66±0.06)%和(1.51±0.15)%,低于Ctrl组的(2.85±0.21)%和(2.05±0.05)%,差异有统计学意义(P<0.05)。与Ctrl组比较,GAL3ST1 OE组Bax降低和Bcl-2、GALC和UGT8蛋白表达增加(P<0.05);GAL3ST1表达上调促进体内肝癌生长,促进Ki-67、PCNA、UGT8和GALC mRNA表达。结论GAL3ST1可能通过参与鞘脂代谢通路调控HCC进展。

粪便脱落细胞BMP3与BCAT1基因甲基化检测对结肠癌及癌前病变筛查的价值

目的分析粪便脱落细胞骨形态发生蛋白3(BMP3)、支链氨基酸氨基转移酶1(BCAT1)甲基化对结肠癌及癌前病变筛查的价值。方法纳入2020年2—12月海南医学院第一附属医院胃肠肿瘤外科患者94例,其中结肠癌患者43例(结肠癌组)、结肠腺瘤患者19例(结肠腺瘤组)、单纯痔疮患者32例(对照组),收集结肠癌患者的临床分期、肿瘤最大径、肿瘤体积、分化程度、淋巴结转移、浸润程度情况;取其粪便样本采用甲基化特异性PCR(MSP)检测粪便脱落细胞BMP3、BCAT1甲基化情况;分析结肠癌患者粪便脱落细胞BMP3、BCAT1及二者联合基因甲基化与临床病理特征关系;受试者工作特征曲线(ROC)评价BMP3、BCAT1单基因及二者联合基因甲基化对结肠腺瘤和结肠癌的诊断价值。结果粪便脱落细胞BMP3、BCAT1单基因及二者联合基因甲基化阳性率比较,结肠癌组>结肠腺瘤组>对照组(χ^(2)/P=18.462/0.000、24.203/0.000、56.039/0.000)。粪便脱落细胞BMP3与BCAT1联合基因甲基化结肠癌患者肿瘤最大径、肿瘤体积大于非甲基化患者(t/P=11.417/0.000、3.381/0.002),分化程度越低、临床分期越高基因甲基化阳性率越高,且高于非甲基化患者(χ^(2)/P=11.646/0.003、4.882/0.027)。粪便脱落细胞BMP3、BCAT1单基因及二者联合基因甲基化对结肠腺瘤诊断的ROC曲线显示,BMP3基因甲基化(AUC=0.579,95%CI 0.433~0.716)、BCAT1基因甲基化(AUC=0.521,95%CI 0.377~0.663)、二者联合基因甲基化(AUC=0.574,95%CI 0.428~0.711),三者AUC比较,差异无统计学意义(Z=0.052,P=0.959)。以上指标对结肠癌诊断的ROC曲线显示,BMP3基因甲基化(AUC=0.701,95%CI 0.585~0.802)、BCAT1基因甲基化(AUC=0.744,95%CI 0.630~0.838)、二者联合基因甲基化(AUC=0.852,95%CI 0.752~0.924),三者AUC比较,BMP3与BCAT1联合基因甲基化的AUC最高(Z=3.598,P=0.000)。结论粪便脱落细胞BMP3、BCAT1甲基化对结肠癌癌前病变筛选价值不大,但对结肠癌有较高的筛选价值,且与结肠癌分化程度、临床分期等关系密切,有一定应用价值。

3,5,2',4'-四羟基查尔酮对小鼠尿酸及尿酸合成相关酶基因的影响

用氧嗪酸钾诱导高尿酸血症动物模型,对化合物3,5,2',4'-四羟基查尔酮(P40)的降尿酸作用及尿酸合成相关酶基因进行研究。用磷钨酸法测定小鼠血清尿酸水平,用RT-PCR测定脑组织中次黄嘌呤鸟嘌呤磷酸核糖转移酶(HGPRT)、肝脏中的磷酸核糖焦磷酸合成酶(PRPS)和磷酸核糖焦磷酸酰胺转移酶(PRPPAT)mRNA的表达水平。结果表明:灌胃给予高尿酸血症小鼠P40 2、4、8 mg/kg和阳性对照药别嘌醇1 mg/kg,共给药5次,每天2次,均显著降低血清尿酸水平(P<0.05,0.01),具有显著的降尿酸作用;但对HGPRT、PRPS、PRPPAT的mRNA表达水平无明显影响。

3-巯基丙酮酸转硫酶在非酒精性脂肪性肝病中对脂肪变性的影响研究

目的探讨3-巯基丙酮酸转硫酶(MPST)在非酒精性脂肪性肝病(NAFLD)中对脂肪变性的影响。方法取20只C57BL/6小鼠,高脂饮食喂养,建立NAFLD模型,分为观察组和对照组(每组10只)。另以10只小鼠予以正常饮食用来参照NAFLD模型的成功建立。观察组小鼠注射重组腺病毒载体shRNA(AD-shRNA)对肝脏MPST进行干预,对照组小鼠注射重组腺病毒载体(AD-GFP)。小鼠处死后取肝组织进行HE染色,观察肝脏脂肪变性情况,并测定肝组织MPST、固醇调节元件结合蛋白-1(SREBP-1)、脂肪酸合成酶(FAS)、胱硫醚γ裂解酶(CSE)表达与肝脏中游离脂肪酸(FFA)、三酰甘油(TG)、总胆固醇(TC)、硫化氢(H2S)的含量。结果观察组小鼠肝脏MPST的mRNA表达水平与对照组相比显著下调,FFA、TG、TC含量与对照组相比也显著降低,差异有统计学意义(P<0.05)。对照组小鼠肝脏内弥漫性肝细胞脂肪变性,且出现肝细胞炎性表现;观察组小鼠肝细胞脂肪变性的弥漫性减轻,炎性肝细胞减少。观察组小鼠肝脏SREBP-1、FAS的mRNA表达水平与对照组相比显著下调,CSE的mRNA表达水平及肝组织H2S含量较对照组显著升高,差异有统计学意义(P<0.05)。结论 H2S在MPST对脂肪肝的调节过程中起主要介导作用,且与SREBP-1相关通路抑制有关。

The GSK3b sensing metabolism controls NLRP3 inflammasome activation

OBJECTIVE To identify the role of GSK3 isoform inhibition on inflammasome activation.METHODS The NLRP3 inflammasome was activated by typical LPS/ATP and host-derived metabolites in primary mouse macrophages.The pharmacological inhibition of GSK3 isoforms on inflammasome activation was assayed by quantifying IL-1βin the supernatant,and activated caspase-1in cell lysates using highly selective inhibitors.Further molecular mechanisms were investigated by protein pulldown assay,confocal imaging using forced gene expression system and endogenous protein tagged mouse macrophages.RESULTS Pharmacological inhibition of GSK3-β,but not GSK3-αisoform suppressed NLRP3 inflammasome activation in response to ATP,urate crystal and the microbial alkaloid toxin staurosporine.GSK3-βinhibition did not inhibit melanoma 2(AIM2)inflammasome activation in response to double-stranded DNA(dsDNA)and did not affect non-canonical caspase-11 inflammasome activation.GSK3-βinhibition suppressed high glucose mediated NLRP3 inflammasome activation.Mechanistically,GSK3-βinhibition blocked NLRP3 inflammasome by preventing pro IL-1βtranscription,reducing caspase-1 activation and ASC speck formation.GSK3-βinhibition blocked NLRP3 inflammasome activation without affecting the level of reactive oxygen species(ROS)which is a crucial component in initialing inflammasome activation.Further studies revealed that GSK3-βdirectly binds to ASC by both co-forced expression and endogenous protein level.Interestingly,we found ASC can be glycosylated in response to inflammasome activation,and GSK3-βinhibition reduced ASC glycosylation.Consistently,the O-Glc NAc transferase(OGT)deficient mouse macrophages showed the significant reduction of mature IL-1βsecretion in response to NLRP3 inflammasome activation.CONCLUSION Our results demonstrate a critical role of metabolism-sensing GSK3-βpathway in mediating NLRP3 inflammasome activation,thus defining a new therapeutic target for sterile inflammation.

琥珀酰辅酶A转移酶的表达纯化及抗体制备

目的:琥珀酰辅酶A转移酶(SCOT)是酮体代谢过程中的关键限速酶,此酶缺陷多由SCOT基因突变引起,患者多有酮症酸中毒表现。为了进一步研究SCOT的功能,采用原核表达系统表达并纯化重组SCOT,制备SCOT多克隆抗体。方法:选择蛋鸡、肉鸡模式生物为研究对象,通过生物信息学对其抗原性和属间同源性进行分析,通过RT-PCR从鸡的骨骼肌cDNA中扩增了SCOT基因N端半长片段,克隆到表达载体pET28b中,在大肠杆菌BL21(DE3)中诱导表达,并用镍离子螯合柱(Ni-NTA)纯化重组SCOT;用纯化的重组SCOT免疫小鼠后得到多克隆抗体。结果:Western印迹表明,制备的SCOT抗体具有较高的特异性,可特异性识别鸡的SCOT蛋白,同时可特异性识别小鼠和人的相应SCOT蛋白。结论:SCOT多克隆抗体的制备为后续在鸡、鼠和人中研究SCOT基因提供基础。

桑叶调节PI3K/Akt/PPARα/CPT-1通路改善2型糖尿病大鼠肝脏糖脂代谢紊乱机制

目的:基于磷脂酰肌醇3-激酶/蛋白激酶B/过氧化物酶体增殖物激活受体α/肉毒碱棕榈酰基转移酶-1(PI3K/Akt/PPARα/CPT-1)信号通路探讨桑叶水提物对2型糖尿病(T2DM)大鼠肝脏糖脂代谢紊乱的作用及其机制。方法:高脂喂养联合腹腔注射链脲佐菌素(STZ)方法制备T2DM模型,按血糖、体质量将造模成功大鼠随机分为模型组、二甲双胍(0.2 g·kg^(-1))组和桑叶水提物(含生药4.0 g·kg^(-1))组,连续给药8周,每周相同时间测定空腹血糖。苏木素-伊红(HE)染色、油红O染色观察肝脏组织形态学和脂肪变化;生化分析法测定血清总胆固醇(TC)、甘油三酯(TG)、低密度脂蛋白胆固醇(LDL-C)、高密度脂蛋白胆固醇(HDL-C)、丙氨酸氨基转移酶(ALT)和天冬氨基酸氨基转移酶(AST)水平;蛋白免疫印迹法(Western blot)检测肝脏磷酸化磷脂酰肌醇3-激酶(p-PI3K)、PI3K、磷酸化蛋白激酶B(p-Akt)、Akt、PPAR-α、CPT-1蛋白表达。结果:给药8周后,与正常组比较,模型组大鼠血糖显著升高(P<0.01);与模型组比较,桑叶水提物组大鼠血糖显著降低(P<0.01)。HE染色显示,正常组大鼠肝组织结构完整,肝细胞以中央静脉为中心呈放射状排列;模型组大鼠肝细胞损伤明显;与模型组比较,桑叶水提物组大鼠空泡变性程度显著降低,未见小胆管增生等病变。油红O染色显示,正常组大鼠肝细胞无明显脂肪变性、坏死,肝细胞几乎无脂滴;模型组大鼠肝内脂滴较正常组明显增加;桑叶给药可明显减少大鼠肝脏脂滴。模型组大鼠TC、TG、LDL-C、AST、ALT水平较正常组显著升高(P<0.01);桑叶水提物组大鼠TC、TG、LDL-C、AST、ALT水平较模型组明显降低(P<0.05,P<0.01)。Western blot结果显示,与正常组比较,模型组大鼠p-PI3K/PI3K、p-Akt/Akt、PPARα和CPT-1的蛋白表达显著降低(P<0.01);与模型组比较,桑叶水提物能明显增加p-PI3K/PI3K、p-Akt/Akt、PPARα和CPT-1的蛋白表达(P<0.05,P<0.01)。结论:桑叶水提物可改善T2DM大鼠肝脏糖代谢紊乱,降糖机制可能与调控PI3K/Akt/PPAR-α/CPT-1信号通路有关。