Exploring the Action Mechanism of Yadanzi(Brucea javanica)in the Treatment of Glioblastoma Based on Bioinformatics and Network Pharmacology

ObjectiveThe aim of the study is to explore the molecular mechanism of Yadanzi(Brucea javanica)in the treatment of glioblastoma(GBM)by using the methods of bioinformatics and network pharmacology.Methods The Traditional Chinese Medicine Systems Pharmacology Database and Analysis Platform(TCMSP)and literature retrieval method were applied to obtain the active ingredients of Yadanzi(Brucea javanica),and to predict the relevant targets of the active ingredients.The GBM-related targets were retrieved and screened through the Gene Expression Profling Interactive Analysis(GEPIA)database,and mapped to each other with the targets of the components of Yadanzi(Brucea javanica)to obtain the intersection targets.The GBM differentially expressed gene targets were imported into the String database to obtain the protein interaction relationship,the Cytoscape software was used to draw the protein interaction network,the Cytobba and MCODE plug-ins were used to screen the core genes and important protein interaction modules,and the GEPIA database was applied to make survival analysis of the core genes.The network map of“active ingredients-targets”was constructed through the Cytoscape 3.6.1 software.Gene Ontology(GO)biological function enrichment analysis and Kyoto Encyclopedia of Genes and Genomes(KEGG)signaling pathway enrichment analysis for GBM differentially expressed genes were performed through the DAVID database.ResultsThrough TCMSP and literature retrieval,23 potential active ingredients and 129 related targets were obtained from Yadanzi(Brucea javanica).In the GEPIA database,247 GBM differentially expressed genes were screened,including 113 upregulated genes and 134 downregulated genes.After mapping with the targets related to the active ingredients of Yadanzi(Brucea javanica),six intersection targets were obtained,that is,the potential action targets of Yadanzi(Brucea javanica)in treating GBM,including MMP2,HMOX1,BIRC5,EGFR,CCNB2,and TOP2A.Cytoscape software was applied to build an“active ingredient-action target”network.Two active ingredients and five action targets of β-sitosterol(BS)and luteolin were found,and the targets were mainly concentrated in BS.It was found by KEGG pathway enrichment analysis that GBM differentially expressed genes were mainly involved in signaling pathways related to Staphylococcus aureus infection,phagosome formation,tuberculosis and systemic lupus erythematosus and other infectious and autoimmune diseases.It was found by GO enrichment analysis that the GBM differentially expressed genes mainly involved such biological processes(BP)as the processing and presentation of exogenous antigenic peptides and polysaccharide antigens through MHC Il molecules,y-interferon-mediated signaling pathways,extracellular matrix composition,and chemical synapses transmission;it involved cellular components such as cell junctions,axon terminal buttons,extracellular space,vesicle membranes for endocytosis,and MHC Il protein complexes;molecular functions such as calcium-mediated ionic protein binding,MHC Il molecular receptor activity,immunoglobulin binding,and phospholipase inhibitor activity were also involved.Survival analysis was conducted by GEPIA on the top 37 core targets in degree value,and a total of five genes related to GBM prognosis were obtained.Among them,FN1 and MMP2 were highly expressed while GABRD(v-aminobutyric acid A receptor delta subunit),RBFOX1,and SLC6A7 were expressed at a low level in cancer patients.Conclusion The pathogenesis of GBM is closely related to the human immune system,and BS and luteolin may be the main material basis of Yadanzi(Brucea javanica)for the treatment of GBM and the improvement of prognosis.The molecular mechanism may be related to the physical barrier formed by destroying the tumor cell stromal 68 Treatment of Glioblastoma Based on Bioinformatics and Network Pharmacology Zhao,Si.molecules and its involvement in tumor immune response.

水芹水醇提取物在雏鸭体内对DHBV-DNA的抑制效果

目的观察水芹(Oenanthe Javanica,OJ)水醇提取物在鸭体内对鸭乙型肝炎病毒(DHBV)-DNA 的抑制效果.方法将 DHBV 感染雏鸭随机分为高、中、低三个剂量组,分别为8,5,3g/kg 组进行药物治疗.每组5～6只,ig,2次/d×10 d;设病毒对照组(DHBV),以生理盐水(NS)代替药物,ig,2次/d×10 d.阳性药用阿昔洛韦(ACV)粉剂250 mg,ig,100mg/kg,2次/d×10 d.在感染7d 后,即用药前(TO),用药后5d(T5),用药10 d(T10)和停药后3 d(P3),自鸭腿胫静脉分别取血,分离血清,检查 DHBV-DNA 水平和肝功能.治疗结束经颈静脉放血处死动物,分别切取雏鸭肝脏,作肝病理检查.结果三批实验结果表明,水芹水醇提取物中,高剂量组对感染雏鸭无毒性,给药5,10 d 能显著降低 DHBV 感染鸭血清DHBV-DNA 水平,即 d5的测定值由1.04分别下降至0.52和0.44,抑制率分别为50.0%和50.6%;d10由0.85分别下降0.42和0.36,抑制率分别为57.7%和57.6%,与病毒对照组比较,均有显著性差异(P<0.05和 P<0.01).低剂量组对鸭血清 DHBV-DNA 也有一定疗效,并显示明显的量效关系.肝功能改善明显,给药10 d,中剂量雏鸭血中 ALT,AST,SB 含量下降率分别为44.1%,44.2%,33.3%.高剂量的下降率分别为61.0%,58.3%,64.4%.低剂量虽对肝功能有改善,但无统计显著性.肝组织病理观察证实,中、高剂量对雏鸭肝脏均有保护作用,肝细胞变性坏死均较轻,肝小叶结构基本完整.结论 OJ 在雏鸭体内有抗 DHBV 的作用,保肝效果显著.

圈养马来穿山甲维生素B缺乏症及其防治初报

本文目的是报道圈养马来穿山甲维生素B缺乏症及防治方法。在华南师范大学穿山甲人工救护与保育研究基地,通过对1例发生后肢运动障碍的圈养马来穿山甲DY14临床症状和死亡后尸体解剖症状观察,结合与DY14具有同样临床症状的个体DY10使用复合维生素B注射液的治疗效果以及提供的人工饲料存在B族维生素缺乏的问题,初步诊断DY10和DY14两个体为维生素B缺乏症。在此基础上,我们讨论了穿山甲对B族维生素的需求,回顾了基地内圈养马来穿山甲类似B族维生素缺乏症的发病情况,认为有必要在原有饲料基础上适当增加B族维生素的含量以预防此类疾病,本文对圈养穿山甲人工饲料改进及B族维生素缺乏症的防治具有重要意义。

水芹总酚酸体外抗HBV作用及其机制探讨

目的观察水芹总酚酸体外对乙型肝炎病毒(HBV)的抑制作用并探讨其作用机制。方法水芹总酚酸对Hep AD38细胞的毒性实验分为水芹总酚酸组(细分为1600、800、400、200、100μg/mL浓度组)和空白对照组。体外培养Hep AD38细胞,用MTT法检测水芹总酚酸的毒性范围。水芹总酚酸体外抗HBV作用实验分为水芹总酚酸组(细分为200、100、50、25μg/mL浓度组)、阳性对照组[恩替卡韦(ETV)10μmol/L]和病毒对照组。用无毒浓度以下的水芹总酚酸药液处理Hep AD38细胞,连续6 d,收取上清和细胞,酶联免疫吸附测定(ELISA)法检测上清中HBsAg、HBeAg滴度;实时荧光定量PCR方法检测细胞内HBV DNA载量。水芹总酚酸对鸭乙型肝炎病毒(DHBV)DNA聚合酶的影响实验分为水芹总酚酸组(细分为400、200、100、50、25μg/mL浓度组)、阴性对照组和DHBV DNA聚合酶对照组。从感染鸭乙肝病毒的鸭肝中提取DHBV DNA聚合酶,分别给予不同浓度水芹总酚酸药液,采用ELISA法检测水芹总酚酸对DHBV DNA聚合酶活性的影响。结果水芹总酚酸对Hep AD38细胞的无毒浓度为400μg/mL。与病毒对照组比较,水芹总酚酸组中的200、100、50μg/mL浓度组的HBsAg、HBeAg滴度和HBV DNA载量均明显降低,差异有高度统计学意义(P<0.01);与DHBV DNA聚合酶对照组比较,水芹总酚酸组中的400、200、100μg/mL浓度组可抑制DHBV DNA聚合酶活性,差异有高度统计学意义(P<0.01)。结论水芹总酚酸体外具有良好的抗HBV作用,其作用机制包括抑制HBV DNA聚合酶的活性。

鸦胆子油乳注射液对结肠炎相关性结直肠癌小鼠的作用及机制研究

目的:建立结肠炎相关性结直肠癌(CAC)小鼠模型,研究鸦胆子油乳注射液(BJOEI)的抗癌作用及机制。方法:将60只SPF级C57BL/6雄性小鼠随机分为正常组、模型组、阿司匹林组和BJOEI低、中、高剂量组,每组10只。除空白组外,各组小鼠均采用氧化偶氮甲烷(AOM)和葡聚糖硫酸钠(DSS)诱导CAC小鼠模型,从第3周开始,各组予以相应药物治疗,阿司匹林组25 mg/kg灌胃,BJOEI低、中、高剂量组分别以1.5 mL/kg、3.0 mL/kg、4.5 mL/kg剂量腹腔注射BJOEI,空白组和模型组腹腔注射等体积生理盐水,1次/d,连续给药10周后取材并记录结直肠肿瘤个数,计算脾脏指数;HE染色观察小鼠的结肠组织病理变化,并进行病理学评分;ELISA法检测小鼠血清白细胞介素(IL)-6水平;免疫组化检测结肠组织Ki67、肿瘤坏死因子(TNF)-α和血管内皮生长因子(VEGF)的表达;Western blot检测结肠组织磷酸化核因子-κB(p-NF-κB)/NF-κB蛋白相对表达量。结果:与模型组相比,BJOEI低、中、高剂量组肠道肿瘤个数和脾脏指数均减少,有统计学意义(P<0.05),肠组织病理学评分和Ki67、TNF-α、VEGF、p-NF-κB/NF-κB表达水平均降低,有统计学意义(P<0.05),BJOEI中、高剂量组血清IL-6水平降低,有统计学意义(P<0.05)。结论:BJOEI可能通过抑制NF-κB通路来减轻肠黏膜炎症反应发挥抗CAC作用。

野生水芹黄酮类物质的提取工艺

采用水浴回流提取法,研究了不同提取剂、提取剂浓度、固液比、提取时间和提取温度对新鲜野生水芹(Oenanthejavanica(Bl.)DC.)中黄酮类物质提取率的影响规律。经正交试验,得到野生水芹黄酮类物质提取工艺的最佳参数为:用90%乙醇于80℃水浴回流提取6h,其中野生水芹叶片料液比为1g∶10mL,叶柄料液比为1g∶5mL。叶片提取率可达2.643mg/g,叶柄提取率可达0.586mg/g。

鸦胆子化学成分研究

从鸦胆子Brucea Javanica(L.)Merr的果实中分离得到活性粗产物,进一步经层析分离得到成分Ⅰ、Ⅱ、Ⅲ,经红外、紫外、核磁共振谱等方法鉴定分别为鸦胆苦醇(Brusatol)、鸦胆因 D(Bruceine D)和鸦胆子甙A(Bruceoside A)。

鸦胆子抗肿瘤活性成分的化学研究

从苦木科植物鸦胆子[Brucea javanica(L.)Merr]干躁果实的硅胶干柱柱层析所得的活性部位中经层析分离得到7个四环三萜苦木内酯成份(A,B,C,D,E,F,G),经UV,IR,~1H-NMR,^(13)C-NMR等方法鉴定分别为鸦胆苦醇(Brusatol A),双氢鸦胆苦醇(Dihydrobrusatol,B),鸦胆因B(Bruceine B,C),鸦胆因D(Bruceine D,D),鸦胆因H(Bruceine H,E),鸦胆子甙A(Bruceoside A,F)和双氢鸦胆子甙A(Yadanzioside A,G)。据报道,鸦胆苦醇和鸦胆子甙A具有较强的抗肿瘤活性。

鸦胆子苷B与肠道菌群相互作用及对人肺癌A549细胞的抑制作用

目的:分析鸦胆子苷B和肠道菌群相互作用,以及其代谢产物对人肺癌A549细胞的抑制活性,探讨鸦胆子苷B对非小细胞肺癌(NSCLC)治疗的价值。方法:采用肠道菌群体外温孵培养法,将鸦胆子苷B与人肠道菌群体外共孵育,通过超高效液相色谱-四极杆-飞行时间串联质谱法(UPLC-Q-TOF-MS)分析代谢转化产物。采用细胞增殖与活性检测法(CCK-8法)检测原型物鸦胆子苷B及其代谢产物对人肺癌A549细胞增殖的影响并计算半数抑制浓度(IC_(50))。取健康雄性大鼠5只,经灌胃给药鸦胆子苷B药液(2 mg·kg^(-1)),连续7 d,分别采集大鼠给药前和给药后的粪便,基于16S rRNA高通量测序分析鸦胆子苷B给药前后肠道菌群变化。结果:鸦胆子苷B可被人肠道菌群经脱糖基水解代谢为鸦胆子苦醇,原型物和转化产物对A549细胞的IC50分别为1755.50、19.57μmol·L^(-1),代谢产物对A549细胞增殖的抑制活性显著优于鸦胆子苷B。肠道菌群分析结果显示,与给药前比较,给药后大鼠肠道菌群α多样性和β多样性未发生明显变化。物种丰度方面,门水平上,鸦胆子苷B降低了放线菌门、变形菌门的物种相对丰度,增加了厚壁菌门、髌骨菌门、蓝细菌门的物种相对丰度;属水平上,鸦胆子苷B降低了葡萄球菌属、气球菌属、嗜冷菌属的物种相对丰度,增加了罗姆布茨菌属、乳杆菌属、狭义梭菌属1、Norank-f-norank-o-Clostridia-UCG-014、苏黎世杆菌属、异杆菌属、糖杆菌念珠菌属的物种相对丰度。功能预测结果显示,与给药前比较,给药后大鼠肠道功能均未发生显著变化。结论:鸦胆子苷B可在肠道菌群作用下脱糖基,转化为苷元鸦胆子苦醇,抗肿瘤活性显著提高。服用鸦胆子苷B不会使肠道菌群结构和功能发生显著变化,造成肠道微生态平衡失调,且给药鸦胆子苷B后出现对NSCLC患者有益的肠道菌群变化。

基于网络药理学和分子对接探讨鸦胆子治疗结直肠癌的作用机制

目的采用网络药理学结合分子对接及体内验证,探究鸦胆子Brucea javanica治疗结直肠癌的活性成分、关键作用靶点及潜在的分子机制。方法从公共数据库中检索并收集鸦胆子的活性成分和对应的靶点以及结直肠癌相关的靶点,通过网络药理学分析出鸦胆子治疗结直肠癌的活性成分、成分-疾病的交集靶点以及可能的信号通路。通过分子对接预测活性成分与靶点蛋白的结合能力。通过体内实验进一步验证鸦胆子活性成分治疗结直肠癌的作用和作用机制。结果在满足筛选条件的15个成分中共筛出鸦胆子苦醇、木犀草素、鸦胆子苷B、β-谷甾醇4个鸦胆子生物活性成分及32个鸦胆子治疗结直肠癌的作用靶点,表皮因子生长受体(epidermal growth factor receptor,EGFR)、半胱氨酸天冬氨酸蛋白酶-3(cysteinasparate protease-3,Caspase-3)及细胞周期蛋白D1(cyclin D1)是鸦胆子治疗结直肠癌的关键靶点,EGFR/磷脂酰肌醇3-激酶(phosphatidylinositol-3-kinase,PI3K)/蛋白激酶B(protein kinase B,Akt)信号通路可能在鸦胆子治疗结直肠癌中发挥重要作用。分子对接结果表示4个生物活性成分均可较好结合,其中鸦胆子苦醇与3个关键靶点的平均结合能负值最大,结合最稳定,可能是鸦胆子抗结直肠癌最有效的活性成分。动物实验结果表明,与对照组比较,鸦胆子苦醇明显抑制裸鼠体内移植瘤的体积和质量(P<0.01),下调肿瘤组织中EGFR、PI3K和Akt的蛋白表达水平(P<0.01),下调与G1/G0期细胞阻滞相关的cyclin D1和细胞周期蛋白依赖性激酶4(cyclin-dependent kinase 4,CDK4)的表达(P<0.01),上调与肿瘤细胞凋亡相关的cleaved Caspase-3表达及B淋巴细胞瘤-2相关X蛋白(B-cell lymphoma-2 associated X protein,Bax)/B淋巴细胞瘤-2(Bcell lymphoma-2,Bcl-2)值(P<0.01),下调与迁移和侵袭相关的蛋白基质金属蛋白酶9(matrix metalloproteinase 9,MMP9)、MMP7表达(P<0.01);鸦胆子苦醇组裸鼠肝功能、肾功能及血液指标均未见显著性差异。结论鸦胆子能够通过多靶点、多通路治疗结直肠癌,其主要活性成分为鸦胆子苦醇,其机制可能与抑制EGFR/PI3K/Akt信号通路从而引起G1/G0期阻滞,抑制增殖、侵袭和迁移,促进细胞凋亡有关。