SD大鼠原代海马神经元的一种优化培养方法

目的建立一种稳定、高效的无血清胎鼠海马神经元原代培养方法,以此来获得纯度更高、活力更好的海马神经元。方法取孕(18±1)d SD大鼠胎鼠海马组织,经消化吹打制成细胞悬液,种植于Neurobasal或DMEM/F12培养基后分为:无血清培养组、胎牛血清培养组、胎牛血清+5-氟-2′脱氧尿苷培养组。3组细胞培养12 h后均全量换液为Neurobasal培养基,FUDR培养组神经元培养至d 3时加入FUDR抑制胶质细胞生长。观察3组海马神经元在不同培养时间点下的生长状态;检测神经元活力、细胞凋亡率以及鉴定海马神经元纯度。结果与胎牛血清培养组相比,无血清培养组培养出来的神经元活力更高,细胞凋亡率低,神经元纯度更高;然而加入FUDR使神经元活力降低,细胞凋亡率增加。结论无血清的培养方法培养出来的神经元活性好,纯度高,且不需要加入胶质细胞抑制剂,是一种可行性较强、较为优化的海马神经元原代培养方法。

复方丹参滴丸对冠心病心绞痛辨证论治疗效影响的Meta分析

目的系统评价复方丹参滴丸联合化学药常规治疗冠心病心绞痛的疗效及安全性。方法检索中文数据库(知网、维普、中国生物医学文献、万方数据)及英文数据库(Pubmed、Cochrane Library)。检索关键词筛选符合条件的研究,根据Cochrane手册评价文献质量,应用Stata13.1和Rev Man 5.3软件进行Meta分析、亚组分析,经上述方法系统性评价复方丹参滴丸治疗冠心病心绞痛在有无辨证用药2种情况下疗效区别。结果纳入39项研究,共计3941例患者,试验组1991例,对照组1 950例,文献质量偏低。Meta分析结果显示,应用化学药常规治疗加用复方丹参滴丸组的临床疗效[RR=1.24,95%CI(1.20,1.28),P<0.00001]、心电图临床疗效[RR=1.29,95%CI(1.21,1.37),P<0.00001]、心绞痛发作频率[WMD=-1.82,95%CI(-3.28,-0.36),P=0.01]、心绞痛发作持续时间[WMD=-2.09,95%CI(-2.67,-1.50),P<0.00001]、超敏C反应蛋白(hs-CRP)[WMD=-2.63,95%CI(-4.39,-0.86),P=0.003]、内皮素(ET)[WMD=-16.22,95%CI(-19.37,-13.06),P<0.000 01]、血小板聚集率[WMD=-7.46,95%CI(-11.15,-3.78),P<0.000 1]、血小板颗粒膜蛋白(GMP-140)[WMD=-5.64,95%CI(-6.88,-4.39),P<0.000 01]、纤维蛋白原[WMD=-0.73,95%CI(-1.00,-0.46),P<0.000 01]与对照组相比有显著差异;在临床疗效方面,辨证用药组与无辨证用药组的合并效应无显著差异(P=0.55,I2=0)。共有15项研究阐述不良反应,试验组有43例出现不良反应,对照组有65例出现不良反应。漏斗图与Egger’s检验结果提示无明显发表偏倚。结论冠心病心绞痛患者应用复方丹参滴丸安全有效,较单纯常规治疗可进一步提高临床疗效。结合辨证论治应用复方丹参滴丸疗效与不辨证用药疗效均显著,且无显著性差异。所得结论仍需建立在更多高质量、大样本量的文献基础上加以论证。

生脉注射液体外对CYP450酶与转运体抑制作用的研究

目的评价生脉注射液对细胞色素P450(cytochrome P450,CYP450)酶与转运体活性的影响。方法根据美国食品和药品管理局(FDA)发布的《药物相互作用研究指导原则(2017)》以及我国发布的《药物相互作用研究技术指导原则(试行)》,在有无生脉注射液的人肝微粒体、人源多药耐药蛋白1(multidrug resistance proteins 1,MDR1)、乳腺癌耐药蛋白(breast cancer resistance protein,BCRP)囊泡和人胚胎肾细胞HEK293中,培养CYP450酶与转运体的探针底物,采用液相色谱-串联质谱联用(LC-MS/MS)及酶标仪检测探针底物代谢产物的生成量或探针底物量,并计算半数抑制浓度(50% concentration of inhibition,IC50)值。结果在30%(体积分数)浓度范围内,生脉注射液对CYP1A2、CYP2B6、CYP2C8、CYP2C9、CYP2C19、CYP2D6、CYP3A4的活性均具有抑制作用,其IC50值分别为6.12%、2.72%、10.00%~30.00%、14.31%、12.96%、12.26%、3.72%。生脉注射液对转运体MDR1、BCRP以及有机阴离子1B1(organic anion transporting polypeptide 1B1,OATP1B1)的活性也具有抑制作用,其IC50值分别为0.15%、0.75%、2.03%。结论生脉注射液可以影响CYP450酶以及转运体活性,与转运体MDR1与BCRP底物联用时,发生药物相互作用的风险较大,临床联用时需监测相关指标或谨慎联用。

Shexiang Baoxin Pill Regulates Intimal Hyperplasia,Migration,and Apoptosis after Platelet-Derived Growth Factor-BB-Stimulation of Vascular Smooth Muscle Cells via miR-451

Objective:To investigate the regulatory roles of Shexiang Baoxin Pill(SXBXW)in neointimal formation and vascular smooth muscle cells(VSMCs)invasion and apoptosis as well as the potential molecular mechanisms using cultured VSMCs model of vascular injury(platelet-derived growth factor(PDGF)-BBstimulated)in vitro.Methods:VSMCs were randomly assigned to 5 groups:blank,PDGF-BB(20 ng/mL+0.1%DMSO),SXBXW-L(PDGF-BB 20 ng/mL+SXBXW low dose 0.625 g/L),SXBXW-M(PDGF-BB 20 ng/mL+SXBXW medium dose 1.25 g/L)and SXBXW-H(PDGF-BB 20 ng/mL+SXBXW high dose 2.5 g/L)group.Cell proliferation was assessed using cell counting kit-8(CCK-8)assay and bromodeoxyuridine(BrdU)incorporation assay,the migration effects were detected by Transwell assay,cell apoptosis rate was measured by the Annexin V/propidium iodide(PI)apoptosis kit.The markers of contractile phenotype of VSMCs were detected with immunofluorescent staining.To validate the effects of miR-451 in regulating proliferation,migration and apoptosis treated with SXBXW,miR-451 overexpression experiments were performed,the VSMCs were exposed to PDGF-BB 20 ng/mL+0.1%DMSO and later divided into 4 groups:mimic-NC(multiplicity of infection,MOI=50),SXBXW(1.25 g/L)+mimic-NC,mimic-miR451(MOI=50),and SXBXW(1.25 g/L)+mimic-miR451,and alterations of proteins related to the miR-451 pathway were analyzed using Western blot.Results:PDGF-BB induced VSMCs injury causes acceleration of proliferation and migration.SXBXW inhibited phenotypic switching,proliferation and migration and promoted cell apoptosis in PDGF-BB-induced VSMCs.In addition,miR-451 was shown to be down-regulated in the VSMCs following PDGF-BB stimulation.SXBXW treatment enhanced the expression of miR-451 in PDGF-BB-induced VSMCs(P<0.05).Compared with SXBXW+mimic-NC and mimicmiR451 groups,the expression of tyrosine 3-monooxygenase/tryptophan 5-monooxygenase activation protein zeta(Ywhaz)and p53 was further reduced in SXBXW+mimic-miR451 group,while activating transcription factor 2(ATF2)was increased in VSMCs(P<0.05).Conclusion:SXBXW regulated proliferation,migration and apoptosis via activation of miR-451 through ATF2,p53 and Ywhaz in PDGF-BB-stimulated VSMCs.