Hypoglycemic mechanism of Tegillarca granosa polysaccharides on type 2 diabetic mice by altering gut microbiota and regulating the PI3K-akt signaling pathwaye

Type 2 diabetes mellitus(T2DM)is a complex metabolic disease threatening human health.We investigated the effects of Tegillarca granosa polysaccharide(TGP)and determined its potential mechanisms in a mouse model of T2DM established through a high-fat diet and streptozotocin.TGP(5.1×10^(3) Da)was composed of mannose,glucosamine,rhamnose,glucuronic acid,galactosamine,glucose,galactose,xylose,and fucose.It could significantly alleviate weight loss,reduce fasting blood glucose levels,reverse dyslipidemia,reduce liver damage from oxidative stress,and improve insulin sensitivity.RT-PCR and Western blotting indicated that TGP could activate the phosphatidylinositol-3-kinase/protein kinase B signaling pathway to regulate disorders in glucolipid metabolism and improve insulin resistance.TGP increased the abundance of Allobaculum,Akkermansia,and Bifidobacterium,restored the microbiota abundance in the intestinal tracts of mice with T2DM,and promoted short-chain fatty acid production.This study provides new insights into the antidiabetic effects of TGP and highlights its potential as a natural hypoglycemic nutraceutical.

Myricetin induces M2 macrophage polarization to alleviate renal tubulointerstitial fibrosis in diabetic nephropathy via PI3K/Akt pathway

BACKGROUND Development of end-stage renal disease is predominantly attributed to diabetic nephropathy(DN).Previous studies have indicated that myricetin possesses the potential to mitigate the pathological alterations observed in renal tissue.Never-theless,the precise molecular mechanism through which myricetin influences the progression of DN remains uncertain.AIM To investigate the effects of myricetin on DN and explore its potential therapeutic mechanism.METHODS Db/db mice were administered myricetin intragastrically on a daily basis at doses of 50 mg/kg or 100 mg/kg for a duration of 12 wk.Subsequently,blood and urine indexes were assessed,along with examination of renal tissue pathology.Kidney morphology and fibrosis were evaluated using various staining techniques including hematoxylin and eosin,periodic acid–Schiff,Masson’s trichrome,and Sirius-red.Additionally,high-glucose culturing was conducted on the RAW 264.7 cell line,treated with 25 mM myricetin or co-administered with the PI3K/Akt inhibitor LY294002 for a period of 24 h.In both in vivo and in vitro settings,quantification of inflammation factor levels was conducted using western blotting,real-time qPCR and ELISA.RESULTS In db/db mice,administration of myricetin led to a mitigating effect on DN-induced renal dysfunction and fibrosis.Notably,we observed a significant reduction in expressions of the kidney injury markers kidney injury molecule-1 and neutrophil gelatinase associated lipocalin,along with a decrease in expressions of inflammatory cytokine-related factors.Furthermore,myricetin treatment effectively inhibited the up-regulation of tumor necrosis factor-alpha,interleukin-6,and interluekin-1βinduced by high glucose in RAW 264.7 cells.Additionally,myricetin modulated the M1-type polarization of the RAW 264.7 cells.Molecular docking and bioinformatic analyses revealed Akt as the target of myricetin.The protective effect of myricetin was nullified upon blocking the polarization of RAW 264.7 via inhibition of PI3K/Akt activation using LY294002.CONCLUSION This study demonstrated that myricetin effectively mitigates kidney injury in DN mice through the regulation of macrophage polarization via the PI3K/Akt signaling pathway.

PI3K/Akt/FoxO1信号通路对人源肺动脉平滑肌细胞及肺动脉高压大鼠细胞凋亡的影响

目的探究磷脂酰肌醇3-激酶(PI3K)/蛋白激酶B(Akt)/叉头框蛋白O1(FoxO1)信号通路对人源肺动脉平滑肌细胞(hPASMC)及肺动脉高压大鼠细胞凋亡的影响。方法细胞实验部分,将hPASMC分为4组:(1)空白对照组;(2)血小板源性生长因子-BB(PDGF-BB)组;(3)PDGF-BB+LY294002组;(4)PDGF-BB+紫杉醇(paclitaxel)组。采用TUNEL检测细胞凋亡,采用蛋白质印迹法检测Bcl-2、裂解的胱天蛋白酶-3(cleaved caspase-3)和PI3K/Akt/FoxO1信号通路相关蛋白表达水平。动物实验部分,将12只SD大鼠随机分为4组:(1)空白对照组;(2)野百合碱(MCT)组;(3)MCT+LY294002组;(4)MCT+paclitaxel组。采用Western blot检测Bcl-2、cleaved caspase-3和PI3K/Akt/FoxO1信号通路相关蛋白表达水平。结果细胞实验部分:相比于PDGF-BB组,PDGF-BB+LY294002组与PDGF-BB+paclitaxel组的Bcl-2表达水平下降(P<0.01),cleaved caspase-3表达水平上升(P<0.01);相比于空白对照组,PDGF-BB+LY294002组与PDGF-BB+paclitaxel组的凋亡率增加(P<0.01)。动物实验部分:相比于MCT组,MCT+LY294002组与MCT+paclitaxel组Bcl-2、磷酸化Akt与磷酸化FoxO1表达水平下降(P<0.01),cleaved caspase-3与FoxO1表达水平上升(P<0.01)。各组之间PI3K表达水平无显著差异。结论PI3K/Akt/FoxO1信号通路抑制hPASMC与肺动脉高压大鼠肺组织的细胞凋亡。

红花提取物通过调节PI3K/Akt/FoxO信号通路改善酒精性肝病

目的探讨红花提取物(Carthamus tinctorius L.extract,CTLE)对酒精诱导的肝损伤小鼠氧化应激、脂质代谢和凋亡水平的影响及其作用机制。方法采用慢性酒精喂养加急性酒精灌胃的酒精性肝病小鼠模型造模。小鼠被随机分为4组,造模期间每天观察小鼠状态变化并记录体质量。造模结束后,收集各组小鼠血液和肝脏组织。对小鼠血液进行生化分析。HE染色和油红O染色进一步评价小鼠肝脏病理损伤程度。应用实时荧光定量PCR(quantitative real-time PCR,qPCR)和Western blot法检测p-PI3K、PI3K、p-Akt、Akt、p-mTOR、mTOR、p-FoxO1、FoxO1、p-FoxO3a、FoxO3a、p-FoxO4、FoxO4、BCL-2和BAX因子的mRNA和蛋白表达水平。结果与模型组相比,CTLE给药组小鼠肝脏病理损伤程度和脂质沉积有所改善;小鼠血清及肝脏中的生化相关指标,如ALT、AST、TG、TC、MDA水平有所降低,GSH、SOD水平有所升高。并且通过调控PI3K/Akt/FoxO通路产生了更多的SOD,减少了活性氧(reactive oxygen species,ROS)对机体的损伤和细胞凋亡。结论CTLE可以通过PI3K/Akt/FoxO通路发挥抗氧化应激和抗凋亡作用,减轻小鼠的酒精性肝损伤,为治疗酒精性肝病和开发相关药物提供新的思路。

Spi1 regulates the microglial/macrophage inflammatory response via the PI3K/AKT/mTOR signaling pathway after intracerebral hemorrhage

Preclinical and clinical studies have shown that microglia and macrophages participate in a multiphasic brain damage repair process following intracerebral hemorrhage.The E26 transformation-specific sequence-related transcription factor Spi1 regulates microglial/macrophage commitment and maturation.However,the effect of Spi1 on intracerebral hemorrhage remains unclear.In this study,we found that Spi1 may regulate recovery from the neuroinflammation and neurofunctional damage caused by intracerebral hemorrhage by modulating the microglial/macrophage transcriptome.We showed that high Spi1expression in microglia/macrophages after intracerebral hemorrhage is associated with the activation of many pathways that promote phagocytosis,glycolysis,and autophagy,as well as debris clearance and sustained remyelination.Notably,microglia with higher levels of Soil expression were chara cterized by activation of pathways associated with a variety of hemorrhage-related cellular processes,such as complement activation,angiogenesis,and coagulation.In conclusion,our results suggest that Spi1 plays a vital role in the microglial/macrophage inflammatory response following intracerebral hemorrhage.This new insight into the regulation of Spi1 and its target genes may advance our understanding of neuroinflammation in intracerebral hemorrhage and provide therapeutic targets for patients with intracerebral hemorrhage.

Downregulation of Serum PTEN Expression in Mercury-Exposed Population and PI3K/AKT Pathway-Induced Inflammation

Objective This study investigated the impact of occupational mercury(Hg) exposure on human gene transcription and expression, and its potential biological mechanisms.Methods Differentially expressed genes related to Hg exposure were identified and validated using gene expression microarray analysis and extended validation. Hg-exposed cell models and PTEN lowexpression models were established in vitro using 293T cells. PTEN gene expression was assessed using qRT-PCR, and Western blotting was used to measure PTEN, AKT, and PI3K protein levels. IL-6 expression was determined by ELISA.Results Combined findings from gene expression microarray analysis, bioinformatics, and population expansion validation indicated significant downregulation of the PTEN gene in the high-concentration Hg exposure group. In the Hg-exposed cell model(25 and 10 μmol/L), a significant decrease in PTEN expression was observed, accompanied by a significant increase in PI3K, AKT, and IL-6 expression.Similarly, a low-expression cell model demonstrated that PTEN gene knockdown led to a significant decrease in PTEN protein expression and a substantial increase in PI3K, AKT, and IL-6 levels.Conclusion This is the first study to report that Hg exposure downregulates the PTEN gene, activates the PI3K/AKT regulatory pathway, and increases the expression of inflammatory factors, ultimately resulting in kidney inflammation.

MicroRNA (let-7b-5p)-targeted DARS2 regulates lung adenocarcinoma growth by PI3K/AKT signaling pathway

Background:The aberrant intraellular expression of a mitochondrial aspartyl tRNA synthetase 2(DARS2)has been reported in human cancers.Nevertheless its critical role and detailed mechanism in lung adenocarcinoma(LUAD)remain unexplored.Methods:Initially,The Cancer Genome Atlas(TCGA)based Gene Expression Profiling Interactive Analysis(GEPIA)database (http:/gepia.cancer-pku.cn/)was used to analyze the prognostic relevance of DARS2 expression in LUAD.Further,cell counting kit(CCK)8,immunostaining,and transwell invasion assays in LUAD cell lines in vitro,as well as DARS2 silence on LUAD by tumorigenicity experiments in wivo in nude mice,were performed.Besides,we analyzed the expression levels of p-PI3K(phosphorylated Phosphotylinosital3 kinase),PI3K,AKT(Protein Kinase B),p-AKT(phosphorylated Protein Kinase B),PCNA(proliferating cell nudear antigen),cleaved-caspase 3,E cadherin,and N-cadherin proteins using the Westem blot analysis.Results:LUAD tissues showed higher DARS2 expression compared to normal tissues.Upregulation of DARS2 could be related to Tumor-Node-Metastasis(TNM)stage,high lymph node metastasis,and inferior prognosis.DARS2 silence decreased the proliferation,migration,and invasion abilities of LUAD cells.In addition,the DARS2 downregulation decreased the PCNA and N-cadherin expression and increased cleaved:caspase 3 and E cadherin expressions in LUAD cells,coupled with the inactivation of the PI3K/AKT signaling pathway.Moreover,DARS2 silence impaired the tumonigenicity of LUAD in vivo.Interestingly,let:7b-5p could recognize DARS2 through a complementary sequence.Mechanistically,the increased let 7b 5p expression attenuated the promo oncogenic action of DARS2 during LUAD progression,which were inversely correlated to each other in the LUAD tssues Conclusion:In summary,let 7b-5p,downregulated DARS2 expression,regulating the progression of LUAD cells by the PI3K/AKT signaling pathway.

COL4A2 enhances thyroid cancer cell proliferation through the AKT pathway

Objectives:Thyroid cancer(THCA)is the most common malignant tumor in endocrine system and the incidence has been increasing worldwide.And the number of patients dying from THCA has also gradually risen because the incidence continues to increase,so the mechanisms related to effective targets is necessary to improve the survival.This study was to preliminarily investigate the effects of the COL4A2 gene on the regulation of thyroid cancer(THCA)cell proliferation and the associated pathways.Methods:Bioinformatics analysis revealed that COL4A2 was closely associated with cancer development.COL4A2 expression in THCA tissues was analyzed using immunohistochemistry,and survival information was determined via Kaplan-Meier curves.The expression of COL4A2 and AKT pathway-related genes were analyzed using qPCR and western blot analyses.Colony formation as well as CCK-8 assays exhibited the cell proliferation level and cell activity,respectively.Downstream of COL4A2 was identified by Gene set enrichment analysis(GSEA).The effects of the COL4A2 and AKT pathways on THCA tumor growth in vivo were determined using a mouse model.Results:Bioinformatics analysis exhibited that COL4A2 plays a significant role in cancer and that the AKT pathway is downstream of COL4A2.THCA patients with high COL4A2 expression had shorter recurrence-free survival.Upregulation of COL4A2 gene expression in 2 THCA cell lines promoted tumor cell growth and activity.The use of AKT pathway blockers also restrained the growth and activity of the 2 THCA cell lines.The use of AKT pathway blockers reduced tumor volume and mass and prolonged mouse survival.Conclusions:COL4A2 can promote the growth as well as development of THCA through the AKT pathway and COL4A2 could be used as a target for THCA.

Alleviatory effect of isoquercetin on benign prostatic hyperplasia via IGF-1/PI3K/Akt/mTOR pathway

We evaluated the effect of isoquercetin(quercetin-O-3-glucoside-quercetin,IQ)as a functional component of Abeliophyllum disistichum Nakai ethanol extract(ADLE)on prostate cell proliferation and apoptosis and its effects on the IGF-1/PI3K/Akt/mTOR pathway in benign prostatic hyperplasia(BPH).Metabolites in ADLE were analyzed using UHPLC-qTOF-MS and HPLC.IQ was orally administered(1 or 10 mg/kg)to a testosterone propionate-induced BPH rat model,and its effects on the prostate weight were evaluated.The effect of IQ on androgen receptor(AR)signaling was analyzed in LNCaP cells.Whether IGF-1 and IQ affect the IGF-1/PI3K/Akt/mTOR pathway in BPH-1 cells was also examined.The metabolites in ADLE were identified and quantified,which confirmed that ADLE contained abundant IQ(20.88 mg/g).IQ significantly reduced the prostate size in a concentration-dependent manner in a BPH rat model,and significantly decreased the expression of AR signaling factors in the rat prostate tissue and LNCaP cells in a concentration-dependent manner.IQ also inhibited the PI3K/AKT/mTOR pathway activated by IGF-1 treatment in BPH-1 cells.In BPH-1 cells,IQ led to G0/G1 arrest and suppressed the expression of proliferation factors while inducing apoptosis.Thus,IQ shows potential for use as a pharmaceutical and nutraceutical for BPH.

灯盏细辛总咖啡酰奎宁酸调控PI3K/Akt/FoxO3a通路延缓衰老的作用机制研究

研究灯盏细辛总咖啡酰奎宁酸(caffeoylquinic acid from Erigeron breviscapus,EBCQA)的抗衰老作用,并探讨其潜在作用机制。以线虫为模型,观察EBCQA对其寿命、氧化抗性、热抗性、运动能力、DAF-16入核、以及超氧化物歧化酶(superoxide dismutase,SOD)、谷胱甘肽过氧化物酶(glutathione peroxidase,GSH-Px)、过氧化氢酶(catalase,CAT)活性和丙二醛(malondialdehyde,MDA)含量的影响。腹腔注射D-半乳糖构建衰老大鼠模型,检测EBCQA对大鼠学习记忆能力、胸腺和脾脏系数、肝脏中磷脂酰肌醇3-激酶(phosphoinositide 3-kinase,PI3K)、蛋白激酶B(Akt/protein kinase B,Akt)、磷酸化Akt(phosphp-Akt,p-Akt)、叉头框蛋白O3a(forkhead box class O3a,FOXO3a)、磷酸化FOXO3a(phosphp-FOXO3a,p-FOXO3a)表达,以及肝脏和血清中SOD、GSH-Px、CAT活性和MDA含量的影响。结果显示,EBCQA能够延长野生型线虫寿命,并提升其氧化抗性、热抗性和运动能力,但对线虫PI3K、Akt、FoxO3a同源体突变株寿命没有显著影响;EBCQA能促进DAF-16入核,通过DAF-16提升线虫的SOD、GSH-Px、CAT活性,降低MDA水平。在D-半乳糖诱导衰老大鼠中,EBCQA给药显著改善大鼠的学习记忆功能,提升胸腺和脾脏系数,降低PI3K、Akt、p-Akt、p-FoxO3a表达和MDA含量,增强SOD、GSH-Px、CAT活性。以上结果表明,EBCQA具有延缓衰老的作用,其机制可能与抑制PI3K和Akt激活、降低FOXO3a磷酸化、促进FOXO3a入核和转录活性、提升抗氧化酶活性和抑制氧化应激相关。

Acalypha australis L.extract inhibits B16 melanoma cell metastasis through PI3K/AKT signaling pathway

Background:Melanoma is a deadly skin tumor resulting from the malignant transformation of melanocytes.It is highly malignant and invasive,with the highest mortality rate among skin cancers.Acalypha australis L.(AAL),a plant with dual medicinal and culinary purposes,is commonly regarded as an edible wild vegetable in southern China.Additionally,AAL has a long history of medicinal use in China,often employed for its hemostatic,anti-diarrheal,and anti-inflammatory properties.Modern pharmacology has demonstrated that AAL possesses functions such as weight loss,antimicrobial activity,antiviral effects,and treatment for ulcerative colitis.However,there is currently no research available regarding its effectiveness and mechanisms of action on melanoma.Methods:In this investigation,we used methyl thiazolyl tetrazolium assay to detect cell viability,transwell assay to detect cell migration and invasion ability,and Western blot assay to detect relevant signaling pathways.Results:The present study reveals that 2 mg/mL AAL effectively suppresses the metastasis of B16 cells,while simultaneously triggering the expression of key apoptosis-related proteins,including Bcl-2,Bax,and cleaved caspased 3.Subsequent investigations demonstrate that AAL exerts this inhibitory effect via the PI3K/AKT signal transduction pathway,as evidenced by the observed deficits in Ras,AKT,p-AKT,and PI3K expression levels.Conclusion:These findings indicated that AAL could be a valuable therapeutic option for reducing the metastatic potential of B16 melanoma cells.

褪黑素通过抑制PTEN/AKT/FOXO3a 通路遏制慢性应激下小鼠卵泡发育不良的机制

目的探究褪黑素通过抑制PTEN/AKT/FOXO3a通路在小鼠卵巢中的激活遏制慢性应激下小鼠卵泡发育不良的机制。方法选取60只6周龄雌性C57BL/6N小鼠,随机分为正常对照组、慢性应激组和褪黑素组,每组各20只。使用实验室称重仪记录小鼠的身体和卵巢的质量。通过酶联免疫吸附试验(enzyme-linked immunosorbent assay,ELISA)试剂盒检测小鼠血清激素水平。通过组织学分析计算小鼠卵巢不同阶段的卵泡数量。通过ELISA和实时定量聚合酶链式反应(real-timefluorescence quantitative polymerase chain reaction,RT-qPCR)检测小鼠血清抗米勒管激素(anti-Müllerianhormone,AMH)的表达。通过蛋白印迹法检测磷脂酰肌醇-3-激酶(phosphatidylinositol-3-kinase)/蛋白激酶B(protein kinase B,AKT)/叉头框转录因子3a(forkhead box transcription factor 3a,FOXO3a)信号通路的表达。通过PCR检测小鼠卵巢PI3K/AKT/FOXO3a的转录水平。统计学方法采用LSD-t检验、χ^(2)检验、单因素方差分析或重复测量资料方差分析。结果慢性应激组与正常对照组的初级卵泡数量[(174±30)个与(107±17)个,t=-148.098]、磷酸化张力蛋白同源物(p-phosphatase tensinhomolog deleted on chromosome ten,p-PTEN)蛋白(2.03±0.19与1.26±0.16,t=-32.207)、p-AKT蛋白(1.99±0.18与1.07±0.05,t=-70.021)、p-FOXO3a蛋白(2.18±0.20与1.18±0.11,t=-64.621)、皮质醇稳定蛋白(cortistatin,CORT)(137±12与83±7,t=-124.235)、促卵泡激素(follicle-stimulating hormone,FSH)[(13.1±1.9)IU/L与(8.2±1.6)IU/L,t=-25.388]比较,慢性应激组水平高于正常对照组(P值均<0.05)。慢性应激组与正常对照组的小鼠身体质量[(22.5±2.5)g与(28.4±4.7)g,t=12.906]、卵巢质量[(9±3)mg与(23±5)mg,t=45.302]、雌二醇水平[(36±8)μg/L与(75±10)μg/L,t=88.937]、雄激素水平[(0.13±0.01)μg/L与(0.20±0.02)μg/L,t=23.123]、促黄体生成素(luteinizing hormone,LH)水平[(3.2±0.3)IU/L与(4.6±0.5)IU/L,t=31.170]以及原始卵泡数量[(87±9)个与(143±27)个,t=111.829]、次级卵泡数量[(92±11)个与(150±21)个,t=130.837]和窦卵泡数量[(43±5)个与(96±8个),t=144.851]比较,慢性应激组低于正常对照组(P值均<0.001)。褪黑素组与慢性应激组的p-PTEN/PTEN(1.15±0.14与2.03±0.19,t=4.983)、p-AKT/AKT(1.21±0.13与1.99±0.18,t=-12.108)、p-FOXO3a/FOXO3a(1.35±0.17与2.18±0.20,t=-11.274)、CORT[(106±10)μg/L与(137±12)μg/L,t=-50.392]和FSH水平[(10.2±1.5)IU/L与(13.1±1.9)IU/L,t=-10.317]比较,褪黑素组低于慢性应激组(P值均<0.001)。褪黑素组与慢性应激组的小鼠身体质量[(26.5±4.1)g与(22.5±2.5)g,t=5.182]、卵巢质量[(17±5)mg与(9±3)mg,t=19.588]、雌二醇水平[(66±6)μg/L与(36±8)μg/L,t=20.485]、雄激素水平[(0.21±0.02)μg/L与(0.13±0.01)μg/L,t=6.458]、LH水平[(4.3±0.4)IU/L与(3.2±0.3)IU/L,t=6.924]以及原始卵泡数量[(125±15)个与(87±9)个,t=38.784]、次级卵泡数量[(137±16)个与(92±11)个,t=29.063]和窦卵泡数量[(76±6)个与(43±5)个,t=49.447]比较,褪黑素组高于慢性应激组(P值均<0.001)。结论褪黑素通过抑制PTEN/AKT/FOXO3a通路成员的磷酸化,升高小鼠血清AMH水平,最终减轻慢性应激诱导的小鼠卵巢原始卵泡丢失和卵泡发育不良。

基于PI3K/Akt/FoxO1通路探讨大黄酸对2型糖尿病大鼠肾损伤的作用

目的 通过PI3K/Akt/FoxO1信号传导通路探讨大黄酸对链脲佐菌素诱导的2型糖尿病大鼠肾脏损伤的作用。方法 通过高脂饮食+小剂量STZ(35 mg/kg)造模,将2型糖尿病大鼠随机分为大黄酸低、高(75、150 mg/kg)剂量组,二甲双胍组(300 mg/kg),模型组,另设正常对照组。连续给药12周后,检测各组大鼠的血糖、体质量、肾脏指数、MDA水平、SOD和GSH-Px活性,HE染色观察各组大鼠肾组织病理形态学改变,Masson三色染色观察胶原表达,免疫组化法与Western blot法检测大鼠肾脏PI3K、Akt与FoxO1蛋白表达。结果 与正常组比较,模型组大鼠体质量、SOD和GSH-Px活性、FoxO1蛋白表达降低(P<0.05),血糖、肾脏指数、肾组织MDA水平和PI3K、Akt蛋白表达升高(P<0.05),肾脏有明显病变损伤;与模型组比较,大黄酸各剂量组体质量、SOD和GSH-Px活性、FoxO1蛋白表达升高(P<0.05),血糖、肾脏指数、肾组织MDA水平和PI3K、Akt蛋白表达降低(P<0.05),肾脏病理损伤得到改善。结论 大黄酸对2型糖尿病大鼠肾脏有保护作用,其机制可能与减轻肾脏氧化应激及调节肾脏PI3K/Akt/FoxO1信号转导通路有关。

miR-21靶向PTEN调控AKT/FoxO1信号通路对胃癌细胞凋亡的机制研究

目的:探究miR-21靶向PTEN调控AKT/FoxO1信号通路对胃癌细胞凋亡的影响。方法:将胃癌SGC-7901细胞分为miR-NC inhibitors组(SGC-7901细胞中转染miR-NC inhibitors质粒)、miR-21 inhibitors组(SGC-7901细胞中转染miR-21 inhibitors质粒)、miR-21 inhibitors+sh-PTEN组(SGC-7901细胞中转染miR-21 inhibitors和sh-PTEN质粒);Control组(不转染任何质粒的SGC-7901细胞)。qRT-PCR检测细胞中miR-21 mRNA表达;采用CCK-8、Transwell小室法和流式细胞仪检测细胞增殖、侵袭能力和凋亡率;蛋白质印迹检测细胞中PTEN、AKT、p-AKT、PI3K、p-PI3K、FoxO1蛋白表达;双荧光素酶报告检测miR-21和PTEN的靶向关系。结果:人正常胃黏膜上皮细胞GES-1(1.00±0.10)相比,胃癌细胞SGC-7901中miR-21(1.89±0.17)表达明显升高(P<0.05)。Control组相比,miR-21 inhibitors组细胞中miR-21表达(0.83±0.10)、增殖率(45.31±4.92)%、侵袭数目(62.34±5.83)个和p-PI3K/PI3K(0.42±0.05)、p-AKT/AKT(0.51±0.05)比值均明显降低,细胞凋亡率(23.48±3.51)%、PTEN(0.98±0.10)和FoxO1(0.76±0.08)蛋白表达明显升高(P<0.0001)。pcDNA-NC组相比,pcDNA-PTEN组细胞增殖率(48.26±5.01)、侵袭细胞数(65.37±6.02)个和细胞中p-PI3K/PI3K(0.46±0.05)、p-AKT/AKT(0.55±0.06)比值均明显降低,细胞凋亡率(25.61±3.27)%及细胞中PTEN(0.91±0.09)和FoxO1(0.70±0.08)蛋白表达升高(P<0.05)。预测发现PTEN的3'UTR端与miR-21有碱基互补结合点位。miR-NC组相比,转染野生型PTEN(PTEN-WT)时miR-21组(0.32±0.03)荧光素酶活性明显降低(P<0.05)。miR-21 inhibitors组相比,miR-21 inhibitors+sh-PTEN组细胞增殖率(90.25±9.14)%和侵袭细胞数(125.69±10.31)个和细胞中p-PI3K/PI3K(0.80±0.08)、p-AKT/AKT(0.76±0.08)比值明显增加,细胞凋亡率(6.24±1.32)和细胞中PTEN(0.30±0.04)、FoxO1(0.38±0.05)蛋白表达降低(P<0.0001)。结论:敲减miR-21可靶向负调控PTEN表达,调控AKT/FoxO1信号通路,抑制胃癌细胞的增殖和侵袭,促进凋亡。

miR-370-3p通过FOXO1/PI3K/AKT通路抑制缺氧/复氧诱导的心肌细胞凋亡

目的探讨微小RNA(miRNA/miR)-370-3p在缺氧/复氧(H/R)H9C2心肌细胞凋亡中的调控作用。方法建立H/R H9C2心肌细胞模型。正常培养的H9C2细胞记为对照组,用miR-370-3p模拟物(miR-370-3p mimic)、miR-370-3p模拟物NC(miR-370-3p mimic NC)不同处理方法处理H/R H9C2心肌细胞。实时荧光定量逆转录聚合酶链反应(quantitative fluorescence of reverse transcription polymerase chain reaction,qRT-PCR)检测细胞中miR-370-3p的表达水平,蛋白质印迹法(Western Blot)检测细胞中Caspase-3、FOXO1、PI3K、AKT、p-PI3K的表达水平,流式细胞术检测细胞的凋亡。结果与对照组相比,H/R组心肌细胞中miR-370-3p的表达下降,miR-370-3p的模拟转染明显增加了miR-370-3p的表达水平。H/R明显促进了H9C2心肌细胞的凋亡,转染miR-370-3p模拟物可明显减轻H9C2心肌细胞的凋亡。H/R处理后,凋亡蛋白caspase-3的水平升高,FOXO1的表达明显增加,p-AKT和p-PI3K的表达明显减少。转染miR-370-3p后,caspase-3与FOXO1的表达明显减少,p-AKT和p-PI3K的表达明显增高。结论miR-370-3p可能通过调控FOXO1/PI3K/AKT的表达抑制H/R诱导的H9C2心肌细胞的凋亡,为改善心肌I/R损伤提供一个新的治疗目标。

miR-217靶向FOXO3影响非小细胞肺癌对吉非替尼耐药性及相关机制

目的检测miR-217对非小细胞肺癌吉非替尼耐药性的影响,并探讨下游靶基因及相关通路。方法qRT-PCR检测人肺正常上皮细胞系BEAS-2B,NSCLC细胞系A549、HCC827、PC9、NCI-H1975及吉非替尼耐药株PC9/GR中miR-217表达量。选取PC9/GR细胞,利用转染技术构建control组、NC-mimic组、miR-217 mimic组、miR-217 mimic+si-NC组、miR-217 mimic+si-FOXO3组细胞,CCK8及克隆形成实验检测细胞增殖能力、流式细胞仪检测细胞凋亡能力,Western blot检测PI3K/AKT信号通路蛋白表达。Targetscan生物信息学网站预测miR-217下游靶基因,双荧光素酶实验检测miR-217与靶基因FOXO3相关性。结果与BEAS-2B相比,miR-217表达量在A549、HCC827、PC9、NCI-H1975细胞中显著降低(P<0.05),随着吉非替尼培养浓度增加,PC9细胞中miR-217基因表达量逐渐降低(P<0.05),并且miR-217在PC9/GR细胞中的表达低于PC9(P<0.05)。相较于control及NC-mimic组,miR-217 mimic组细胞增殖能力明显降低(P<0.05),细胞凋亡数量增多(P<0.05),p-PI3K和p-AKT蛋白表达量降低(P<0.05)。双荧光素酶报告表明FOXO3是miR-217的靶标。回复实验测得,与miR-217 mimic组及miR-217 mimic+si-NC组相比,miR-217 mimic+si-FOXO3组细胞耐药能力升高(P<0.05),增殖能力显著提升(P<0.05),细胞凋亡数量减少(P<0.05),p-PI3K和p-AKT蛋白表达量增高(P<0.05)。结论miR-217过表达逆转NSCLC细胞PC9/GR对吉非替尼的耐药性并抑制PC9/GR细胞增殖加速凋亡,这种机制可能与靶向FOXO3调控PI3K/AKT信号通路相关。

基于PI3K/AKT1/FoxO3a信号通路探讨蛭龙活血通瘀胶囊对糖尿病心肌病大鼠的影响

目的:探讨蛭龙活血通瘀胶囊对糖尿病心肌病大鼠的影响及其可能的作用机制。方法:将40只SD大鼠随机分为正常对照组、模型组、蛭龙活血通瘀胶囊组、二甲双胍组,使用高脂饲料及腹腔注射链脲佐菌素的方法建立糖尿病心肌病模型。给药8 w后取材,检测血清GHb、TC、TG、LDL-C、HDL-C的水平;采用HE染色、Masson染色和TUNEL染色分别观察大鼠心肌组织病理学改变、胶原沉积及细胞凋亡情况;采用RT-PCR检测各组大鼠心肌组织PI3K、AKT1、FoxO3a mRNA表达;采用Westerm Blot检测各组大鼠心肌组织p-PI3K、p-AKT1、p-FoxO3a蛋白表达。结果:与正常对照组比较,模型组大鼠血清GHb、TC、TG、LDL-C水平及心肌细胞凋亡率显著升高,心肌组织PI3K、AKT1、FoxO3a mRNA及p-PI3K、p-AKT1、p-FoxO3a蛋白表达显著降低(P<0.01),HDL-C差异无统计学意义(P>0.05)。与模型组比较,蛭龙活血通瘀胶囊组血清GHb、TC、TG、LDL-C水平及心肌细胞凋亡率显著降低,血清HDL-C水平和心肌组织PI3K、AKT1、FoxO3a mRNA及p-PI3K、p-AKT1、p-FoxO3a蛋白表达显著升高(P<0.05或P<0.01);病理染色结果显示模型组心肌纤维肥大,排列紊乱,可见少量炎性细胞浸润,部分区域可见弥漫性的纤维蓝染及坏死细胞,经治疗后细胞肥大、纤维蓝染及坏死情况明显改善。结论:蛭龙活血通瘀胶囊可通过上调心肌组织PI3K、AKT1、FoxO3a mRNA表达及其蛋白的磷酸化有效降低糖尿病心肌病大鼠GHb及血脂,抑制心肌纤维化和心肌细胞凋亡。

丹栀调脂汤对高脂诱导MAFLD大鼠PI3K/AKT/FOXO1信号通路的影响

目的研究丹栀调脂汤对高脂饮食诱导的代谢相关脂肪性肝病(MAFLD)大鼠PI3K/AKT/FOXO1信号通路的影响,探讨其在MAFLD治疗中的作用。方法雄性SD大鼠分为正常组、模型组及丹栀调脂汤高、中、低剂量组。正常组和模型组予等体积的生理盐水,丹栀调脂汤高、中、低剂量组分别予丹栀调脂汤20.4、10.2、5.1 g·kg^(-1)·d^(-1),连续灌胃8周后取材。检测5组大鼠体质量、血脂、血糖、胰岛素水平及HOMA-IR变化情况;肝脏组织脂质沉积情况;Western blot检测PI3K/AKT信号通路中各蛋白表达水平。结果与正常组比较,模型组大鼠体质量、TG、TC、FFA、GLU、INS、LDL-C及HOMA-IR水平明显升高,HDL-C水平明显降低;肝脏组织油红O染色可见明显肿大的肝细胞及明显的脂质沉积;PI3K、AKT蛋白磷酸化表达水平显著降低。相较于模型组,丹栀调脂汤高、中、低剂量组体质量、TG、TC、FFA、GLU、INS、LDL-C及HOMA-IR水平不同程度降低;肝细胞肿大、肝细胞脂滴及排列结构均有不同程度的改善;PI3K、AKT、FOXO1蛋白磷酸化表达水平升高。结论丹栀调脂汤可能通过PI3K/AKT/FOXO1信号通路改善胰岛素抵抗,进而达到防治MAFLD的目的。

芍药苷通过调控Akt/FoxO1信号通路对2型糖尿病大鼠的保护作用

目的探讨芍药苷对2型糖尿病(T2DM)大鼠的作用。方法高糖高脂饮食加注射链脲佐菌素(STZ)法建立T2DM大鼠模型,并随机分为模型组、二甲双胍组(100 mg/kg)和芍药苷高、低剂量组(200、100 mg/kg),每组10只,另选10只健康大鼠作为正常组,各组灌胃给予相应剂量药物,每天1次,持续8周。给药第7周进行葡萄糖耐量实验,给药结束后使用试剂盒检测空腹血糖(FBG)、空腹胰岛素(FINS)、胰岛素抵抗指数(IRI)及血清高密度脂蛋白胆固醇(HDL-C)、低密度脂蛋白胆固醇(LDL-C)、总胆固醇(TC)、甘油三酯(TG)水平,HE染色观察肝组织病理形态,ELISA法检测肝组织白细胞介素1β(IL-1β)、肿瘤坏死因子α(TNF-α)、白细胞介素6(IL-6)、丙二醛(MDA)水平和谷胱甘肽过氧化物酶(GSH-Px)、过氧化氢酶(CAT)活性,Western blot法检测肝组织蛋白激酶B(Akt)、叉头状转录因子O1(FoxO1)蛋白表达。结果与模型组比较,二甲双胍组和芍药苷各剂量组大鼠FBG、FINS、IRI均降低(P<0.01),葡萄糖耐受能力得到改善;血清HDL-C水平升高(P<0.05,P<0.01),LDL-C、TC和TG水平降低(P<0.05,P<0.01),肝组织病理性损伤减轻;肝组织IL-1β、TNF-α和IL-6水平降低(P<0.05,P<0.01);肝组织MDA水平和p-Akt蛋白表达降低(P<0.05,P<0.01),肝组织GSH-Px、CAT活性和p-FoxO1蛋白表达升高(P<0.05,P<0.01)。结论芍药苷具有改善2型糖尿病大鼠糖脂代谢紊乱,抑制炎症反应及氧化应激的作用。

How is the AKT/mTOR pathway involved in cell migration and invasion?

As a pathway that plays a role in nutrient absorption,anabolic response,cell growth and survival,the important role of AKT/mTOR in tumorigenesis has also come to light.For cancer patients,most deaths are caused by the growth of metastatic tumors outside the primary focus.Therefore,migration and invasion in the late stage of tumor progression are the main unresolved issues in the study of tumor pathogenesis,and AKT/mTOR has been found to participate in the migration and invasion of cancer cells,which means that the study of this pathway may contribute to a solution for the problem.Because of its extensive and complex functions in the organism,this pathway can be regulated by a variety of different signals in the body,and then realize its function through different downstream signal molecules.This article reviews the proteins that can indirectly affect this pathway by regulating the common upstream signaling molecules of this pathway,and the proteins that can directly affect the level of phosphorylation of AKT/mTOR in cancer cells.We also review the proteins that can co-regulate this pathway and its downstream pathways.Through this study,we hope to gain a deeper understanding of the regulatory mechanism of the AKT/mTOR pathway in cancer cells,in hopes of finding effective and harmless cancer treatment targets in the future.