Combining cytochrome P-450 3A4 modulators and cyclosporine or everolimus in transplantation is successful

AIM: To describe the long term follow-up of kidney allograft recipients receiving ketoconazole with calcineurin inhibitors(CNI) alone or combined with everolimus. METHODS: This is an open-label, prospective observational clinical trial in low immunologic risk patients who, after signing an Institutional Review Board approved consent form, were included in one of two groups. The first one(n = 59) received everolimus(target blood level, 3-8 ng/m L) and the other(n = 114) azathioprine 2 mg/kg per day or mycophenolate mofetyl(MMF) 2 g/d. Both groups also received tapering steroids, the cytochrome P-450 3A4(CYP3A4) modulator, ketoconazole 50-100 mg/d, and cyclosporine with C0 targets in the everolimus group of 200-250 ng/mL in 1 mo, 100-125 ng/m L in 2 mo, and 50-65 ng/m L thereafter, and in the azathioprine or MMF group of 250-300 ng/mL in 1 mo, 200-250 ng/mL in 2 mo, 180-200 ng/m L until 3-6 mo, and 100-125 ng/mL thereafter. Clinical visits were performed monthly the first year and quarterly thereafter by treating physicians and all data was extracted by the investigators.RESULTS: The clinical characteristics of these two cohorts were similar. During the follow up(66 + 31 mo), both groups showed comparable clinical courses, but the biopsy proven acute rejection rate during the full follow-up period seemed to be lower in the everolimus group(20% vs 36%; P = 0.04). The everolimus group did not show a higher surgical complication rate thanthe other group. By the end of the follow-up period, the everolimus group tended to show a higher glomerular filtration rate. Nevertheless, we found no evidence of a consistent negative slope of the temporal allograft function estimated by the modification of the diet in renal disease formula in any of both groups. At 6 years of follow-up, the uncensored and death-censored graft survivals were 91% and 93%, and 91% and 83% in the everolimus plus cyclosporine, and cyclosporine alone groups, respectively. The addition of ketoconazole saved 80% of cyclosporine and 56% of everolimus doses. CONCLUSION: Combining CYP3A4 modulators with CNI or mammalian target of rapamycin inhibitor, in low immunological risk kidney transplant recipients is feasible, effective, safe and affordable even in the long term.

注射用丹参总酚酸(冻干)对人CYP450酶和P-糖蛋白体外抑制作用及对大鼠CYP1A2和CYP3A体内诱导作用(英文)

目的探讨注射用丹参总酚酸(冻干)(SLI)对人CYP450酶和P-糖蛋白体外抑制作用以及对大鼠CYP1A2和CYP3A体内诱导作用。方法①应用P450-GloTMCYP450检测试剂盒,通过化学发光法测定SLI和经典抑制剂对细胞色素P4501A2(CYP1A2),CYP2D6,CYP3A4,CYP2C19和CYP2C9的IC50值,通过比较SLI和经典抑制剂对相应细胞色素P450亚型的IC50值来判断SLI对人CYP450酶的体外抑制作用。②Wistar大鼠分别iv给予SLI 3,10和30 mg·kg-1和诱导剂苯巴比妥钠20 mg·kg-1,采用探针底物法,通过比较代谢产物的生成速率来评价SLI对大鼠CYP1A2和CYP3A的诱导作用。③应用ATP酶检测试剂盒,通过化学发光法测定ATP酶活性来评价SLI是否为P-gp的底物或抑制剂。结果①CYP1A2,CYP2C9,CYP2C19,CYP2D6和CYP3A4抑制剂的IC50与SLI对其的IC50进行比较(CYP1A2:0.12μmol·L-1vs 840μmol·L-1;CYP2C9:3.362μmol·L-1vs 704μmol·L-1;CYP2C19:3.236μmol·L-1vs 306μmol·L-1;CYP2D6:0.117μmol·L-1vs 2660μmol·L-1;CYP3A4:0.078μmol·L-1vs 1780μmol·L-1)。②与空白对照组(86.4±6.3)nmol·g-1.min-1相比,SLI 3,10和30 mg·kg-1组CYP1A2活性分别为83.4±6.6,82.5±4.0和(83.4±6.6)nmol·g-1.min-1。与空白对照组(16.1±0.9)nmol·g-1.min-1比较,SLI 3,10和30 mg·kg-1组CYP3A活性分别为15.7±0.6,15.9±0.7和(15.9±1.0)nmol·g-1.min-1,无显著性差异。③以临床血药浓度为依据设计的一系列浓度的SLI 0.0002,0.0006,0.002,0.006,0.017,0.052,0.156和0.468 g.L-1的ATP酶活性分别与空白对照组进行比较(5.8,5.3,5.8,5.5,5.8,5.2,,5.8,5.3,vs 5.75μmol·g-1.min-1),无显著性差异。结论SLI临床给药剂量既不能体外抑制人CYP1A2,CYP2D6,CYP3A4,CYP2C19和CYP2C9酶活性,也不能诱导大鼠CYP1A2和CYP3A,同时也不是P-gp的体外抑制剂或底物。

In vitro and in vivo cytochrome P450 3A enzyme inhibition by Aframomum melengueta and Dennettia tripetala extracts

Objective: To evaluate the in vitro and in vivo inhibitory effects of two commonly used herbs, Aframomum melengueta(A. melengueta) and Dennettia tripetala(D. tripetala) on CYP 3A enzymes. Methods: In vitro inhibition of the enzymes were assessed with microsomes extracted from female albino rats using erythromycin-N-demethylation assay(EMND) method while their in vivo effects were measured by estimating simvastatin plasma concentrations in rats. Pharmacokinetic parameters were determined using non-compartmental anaysis as implemented in Win Nonlin pharmacokinetic program. Results: EMND assay with intestinal microsomes indicated that aqueous extracts of D. tripetala and A. melengueta significantly(P < 0.05) inhibited intestinal CYP 3A activity at both 50 μg and 100 μg concentrations. Petroleum ether extract of D. tripetala and ethanol extracts of A. melengueta inhibited intestinal CYP3 A activity at 100 μg but not at 50 μg concentrations. All the extracts showed an in vitrodose dependent CYP 3A inhibition with liver microsomes. In vivo analysis showed that pretreatment with the extracts enhanced systemic absorption of simvastatin with reductions in metabolizing enzymes activity as indicated in significant increases in maximal concentration, area under curve, area under moment curve and mean resident time of simvastatin(P < 0.05). Conclusions: Herbal preparations containing these plants' extracts should be used with caution especially in patients on CYP450 3A substrate medications.

cAMP-PKA信号通路对L02细胞药物代谢酶CYP3A的调控作用

目的探讨cAMP-PKA信号通路对细胞色素P4503A(CYP3A)在正常肝细胞L02表达中的作用。方法 L02细胞中分别加入8-溴-环腺苷酸(8-Br-cAMP)10μmol.L-1及抑制剂H-89 10μmol.L-1,培养48 h,分别采用完整细胞免疫组化法、Western印迹法和红霉素-N-脱甲基法检测细胞中PKA、孕烷X受体(PXR)及CYP3A的表达。结果与正常对照组PKA蛋白表达(211±20)、PXR蛋白表达(0.45±0.14)及CYP3A的活性〔(0.38±0.02)μmol.min-1.g-1蛋白〕相比,8-Br-cAMP 10μmol.L-1处理后,细胞PKA蛋白表达(296±18)升高、PXR蛋白表达(0.69±0.21)升高、CYP3A的活性〔(0.43±0.01)μmol.min-1.g-1蛋白〕增强;H-89 10μmol.L-1处理后细胞中PKA蛋白表达(176±14)降低,PXR蛋白表达(0.47±0.13)及CYP3A的活性〔(0.39±0.05)μmol.min-1.g-1〕减弱,无统计学差异。结论 cAMP-PKA信号通路可能是药物代谢酶CYP3A的调控途径之一。

Cytochrome P450 2E1 genetic polymorphism and gastric cancer in Changle,Fujian Province

AIM: Genetic polymorphism in enzymes of carcinogen metabolism has been found to have the influence on the susceptibility to cancer. Cytochrome P450 2E1 (CYP2E1) is considered to play an important role in the metabolic activation of procarcinogens such as N-nitrosoamines and low molecular weight organic compounds. The purpose of this study is to determine whether CYP450 2E1 polymorphisms are associated with risks of gastric cancer. METHODS: We conducted a population based case-control study in Changle county, Fujian Province, a high-risk region of gastric cancer in China. Ninety-one incident gastric cancer patients and ninety-four healthy controls were included in our study. Datas including demographic characteristics, diet intake, and alcohol and tobacco consumption of individuals in our study were completed by a standardized questionnaire.PCR-RFLP revealed three genotypes:heterozygote (C1/C2) and two homozygotes (C1/C1 and C2/C2) in CYP2E1. RESULTS: The frequency of variant genotypes (C1/C2 and C2/C2) in gastric cancer cases and controls was 36.3% and 24.5%, respectively. The rare homozygous C2/C2 genotype was found in 6 individuals in gastric cancer group(6.6%), whereas there was only one in the control group (1.1%). However, there was no statistically significant difference between the two groups (two-tailed Fisher's exact test P=0.066). Individuals in gastric cancer group were more likely to carry genotype C1/C2 (odds ratio, OR=1.50) and C2/C2 (OR=7.34) than individuals in control group (chi(2) =4.597, for trend P=0.032). The frequencies of genotypes with the C2 allele (C1/C2 and C2/C2 genotypes) were compared with those of genotypes without C2 allele (C1/C1 genotype) among individuals in gastric cancer group and control group according to the pattern of gastric cancer risk factors. The results show that individuals who exposed to these gastric cancer risk factors and carry the C2 allele seemed to have a higher risk of developing gastric cancer. CONCLUSION: Polymorphism of CYP2E1 gene may have some effect in the development of gastric cancer in Changle county, Fujian Province.

Three new alternative splicing variants of human cytochrome P450 2D6 mRNA in human extratumoral liver tissue

AIM: To identify the new alternative splicing variants of human CYP2D6 in human extratumoral liver tissue with RT-PCR and sequencing. METHODS: Full length of human CYP2D6 cDNAs was amplificated by reverse transcription-polymerase chain reaction (RT-PCR) from a human extratumoral liver tissue and cloned into pGEM-T vector. The cDNA was sequenced. Exons from 1 to 4 of human CYP2D6 cDNAs were also amplificated by RT-PCR from extratumoral liver tissues of 17 human hepatocellular carcinomas. Some RT-PCR products were sequenced. Exons 1 to 4 of CYP2D6 gene were amplified by PCR from extratumoral liver tissue DNA. Two PCR products from extratumoral liver tissues expressing skipped mRNA were partially sequenced. RESULTS: One of the CYP2D6 cDNAs had 470 nucleotides from 79 to 548 (3' portion of exons 1 to 5' portion of exon 4), and was skipped. Exons 1 to 4 of CYP2D6 cDNA were assayed with RT-PCR in 17 extratumoral liver tissues. Both wild type and skipped mRNAs were expressed in 4 samples, only wild type mRNA was expressed in 5 samples, and only skipped mRNA was expressed in 8 samples. Two more variants were identified by sequencing the RT-PCR products of exons 1 to 4 of CYP2D6 cDNA. The second variant skipped 411 nucleotides from 175 to 585. This variant was identified in 4 different liver tissues by sequencing the RT-PCR products. We sequenced partially 2 of the PCR products amplified of CYP2D6 exon 1 to exon 4 from extratumoral liver tissue genomic DNA that only expressed skipped mRNA by RT-PCR. No point mutations around exon 1, intron 1, and exon 4, and no deletion in CYP2D6 gene were detected. The third variant was the skipped exon 3, and 153 bp was lost. CONCLUSION: Three new alternative splicing variants of CYP2D6 mRNA have been identified. They may not be caused by gene mutation and may lose CYP2D6 activity and act as a down-regulator of CYP2D6.

CYP3A4^＊ 1G、CYP3A5^＊ 3基因多态性对肾移植后高血压患者他克莫司血药浓度/剂量比的影响

目的：探讨肾移植后高血压患者中CYP3A4^＊1G、CYP3A5^＊3基因多态性对他克莫司血药浓度/剂量比（C/D）的影响。方法：以70例肾移植后高血压患者为研究对象,使用PCRRFLP法和测序法检测患者CYP3A4^＊1G、CYP3A5^＊3基因型,患者连续服用他克莫司至少达3 d后,采用微粒子酶免疫分析法（MEIA）测定患者的他克莫司血药谷浓度（C0）,比较CYP3A4^＊1G和CYP3A5^＊3基因多态性对患者他克莫司血药浓度/剂量比（C/D）的影响。结果：肾移植后高血压患者中,携带CYP3A4^＊1G野生型（^＊1^＊1）患者的他克莫司C/D明显高于CYP3A4突变杂合子（^＊1^＊1G）和CYP3A4突变纯合子（^＊1G^＊1G）携带者（P〈0.05）;CYP3A5^＊3突变纯合子（^＊3^＊3）患者的他克莫司C/D明显高于CYP3A5野生型（^＊1^＊1）和CYP3A5突变杂合子（^＊1^＊3）基因型患者（P〈0.05）。要达到相同的目标血药浓度,CYP3A4^＊1G的^＊1^＊1G和^＊1G^＊1G患者比^＊1^＊1患者需要更高剂量的他克莫司,CYP3A5^＊3的^＊1^＊1和^＊1^＊3患者比^＊3^＊3患者需要更高剂量的他克莫司。结论：CYP3A4^＊1G、CYP3A5^＊3基因多态性与肾移植后高血压患者的他克莫司C/D显著相关。

CYP3A5基因多态性指导他克莫司治疗重症肌无力的初步探讨

目的比较他克莫司(FK506)治疗FK506不同代谢型重症肌无力(MG)患者的疗效、有效血药浓度、有效剂量及安全性的差异,并初步探讨CYP3A5基因多态性在指导MG个体化治疗中的作用。方法收集MG患者32例,行CYP3A5*3A6986G等位基因多态性检测,AA型及AG型归为快代谢型组,GG型为慢代谢型组。均给予FK506 0.5～1mg/d口服,逐渐加量,每天记录患者绝对评分,当与治疗前相比绝对评分减少大于50%时,为治疗达标,记录当时的剂量、总服药天数及血药浓度。结果达标时快代谢组的平均血药浓度/剂量(C/D)明显低于慢代谢组(P<0.01),当时口服的FK506剂量/体重也明显大于慢代谢组(P<0.01),达标时间也明显长于慢代谢组(P<0.05),治疗期间共出现3例(9.4%)轻度不良反应。结论 FK506治疗不同CYP3A5*3基因型MG患者的起效时间、有效剂量、有效血药浓度均不同;CYP3A5基因多态性检查在FK506个体化治疗MG中具有一定指导意义。

五酯胶囊联合他克莫司在CYP3A5基因表达型重症肌无力患者治疗中的临床应用

目的探讨五酯胶囊对重症肌无力(MG)患者他克莫司(FK506)血药浓度及临床疗效的影响,并进行用药成本及安全性评估。方法采用双向队列研究方法,纳入2018年2月至2020年5月于北京医院神经内科应用他克莫司治疗的MG住院患者共85例,患者均为CYP3A5基因表达型(AA、AG型)。根据是否联用五酯胶囊将患者分为联合组(FK506+五酯胶囊,n=41例)和单药组(单用FK506,n=44例),对患者进行随访至少2年。比较两组患者FK506临床起效时间、FK506年均血药浓度、日均使用剂量、日均费用及临床疗效的差异,并评估相关副作用。结果联合组临床起效时间明显短于单药组〔(13.14±3.30)d比(20.45±3.92)d;P<0.01〕;1年内FK506年均血药浓度〔(10.03±1.36)ng/mL比(4.78±1.71)ng/mL〕、许氏评分改善率〔M d(Q):92.0%(51.00%)比45.5%(28.75%)〕明显高于单药组(均P<0.01),日均FK506使用剂量〔(2.10±0.703)mg比(3.83±0.976)mg〕、日均费用〔(34.71±11.27)元比(61.27±15.62)元〕、许氏临床绝对评分〔M d(Q):1.00(3.50)分比5.00(9.75)分〕明显低于单药组(均P<0.01);用药2年后两组患者血糖、血脂、肌酐、尿酸异常率无显著统计学差异(均P>0.05),联合组临床痊愈比例(92.7%比72.7%)、停用溴吡斯的明比例(73.2%比11.4%)、FK506减药者比例(17.1%比2.3%)明显高于单药组(P<0.05或P<0.01)。结论五酯胶囊可缩短CYP3A5基因表达型MG患者FK506临床起效时间,提高FK506血药浓度,降低FK506日均使用剂量,明显降低治疗成本,并显著提高临床治疗效果,且未增加FK506的副作用。五酯胶囊为临床应用FK506治疗MG的有效增效剂及费用节省剂。

姜黄素对酒精性肝损伤大鼠CYP3A的影响及机制探讨

目的探究姜黄素对酒精性肝损伤(ALD)大鼠细胞色素P450 3A(CYP3A)的影响及其机制。方法 60只建模成功的ALD大鼠按随机数字表法分为模型组,姜黄素低、中、高剂量组(分别灌胃40、80、160 mg/kg姜黄素)及阳性对照组(腹腔注射200 mg/kg腺苷蛋氨酸),每组12只;对照组12只正常饲养,灌胃等体积生理盐水,连续6周。全自动生化分析仪检测血清中丙氨酸转氨酶(ALT)、天冬氨酸转氨酶(AST)和碱性磷酸酶(ALP)水平;苏木精-伊红(HE)染色观察肝脏形态变化;荧光定量聚合酶链反应(q PCR)检测肝脏组织中孕烷X受体(PXR)、组成型雄甾烷受体(CAR)、CYP3A25 mRNA水平;Western blot检测肝脏组织中PXR、CAR蛋白水平。以大鼠原代肝细胞为研究对象,分别用0、100、200、300、400、500 mmol/L乙醇培养细胞,取细胞增殖抑制率约为50%时的乙醇浓度进行下一步实验;0、0.5、1.0、2.0、4.0、8.0、16.0μmol/L姜黄素培养细胞,取最适姜黄素浓度进行后续研究。实验分为对照组、乙醇组、姜黄素组、姜黄素+siRNA-NC组及姜黄素+siRNA-CYP3A25组。CCK-8检测细胞增殖情况;qPCR检测细胞中CYP3A25 mRNA水平;Western blot检测细胞中PXR、CAR蛋白水平。结果动物实验:与对照组相比,模型组血清中ALT、AST、ALP水平升高(P<0.05);与模型组相比,姜黄素低剂量组血清中ALT、ALP水平降低,肝脏组织中PXR、CAR mRNA和蛋白,CYP3A25 mRNA水平升高(P<0.05),姜黄素中、高剂量组血清中ALT、AST、ALP水平降低,肝脏组织中PXR、CAR mRNA和蛋白,CYP3A25 mRNA水平升高(P<0.05);随着剂量升高,各指标逐渐恢复。细胞实验:与对照组相比,乙醇组细胞增殖抑制率升高(P<0.05),细胞中PXR、CAR蛋白水平降低(P<0.05);与乙醇组相比,姜黄素组细胞增殖抑制率降低(P<0.05),细胞中CYP3A25 mRNA,PXR、CAR蛋白水平升高(P<0.05);与姜黄素组相比,姜黄素+siRNA-CYP3A25组细胞增殖抑制率升高(P<0.05),细胞中CYP3A25 mRNA,PXR、CAR蛋白水平降低(P<0.05)。结论姜黄素可上调CYP3A25水平,促进药物代谢,实现对ALD的缓解,这一过程可能与升高PXR、CAR表达有关。

人体内细胞色素P450 3A探针的研究进展

人体内细胞色素P450 3A(CYP3A)是细胞色素P450酶系中最主要的一类。评价CYP3A的活性可用于研究药动学、药物或毒物的代谢、药物相互作用、药物代谢酶的遗传多态性及疾病与代谢酶的相互影响,从而预测最佳给药剂量,达到提高药物治疗效果和减少不良反应的目的。评价CYP3A的活性一般采用探针法,其评价结果的优劣取决于探针的特异性、安全性和方法的科学性。本文就目前被广泛应用的几种CYP3A探针的研究进展作一综述和评价。

CYP3A4高表达肝细胞株建立及其对三氯乙烯毒性的影响

目的建立CYP3A4高表达肝细胞株并观察其对三氯乙烯毒性的影响。方法 PCR扩增CYP3A4基因并将其克隆到慢病毒高表达载体中,将已经构建的慢病毒载体进行转染后,收集病毒上清,感染正常L02肝细胞。用嘌罗霉素进行筛选得到CYP3A4高表达肝细胞株,通过荧光定量PCR和Western蛋白质印迹法鉴定细胞株。用三氯乙烯0,0.25,0.5,1.0,2.0和4.0mmol·L-1对正常肝肝细胞和CYP3A4高表达肝细胞进行染毒12h,实时定量PCR检测凋亡基因bcl-2,胱天蛋白酶3,胱天蛋白酶8和胱天蛋白酶9以及癌基因c-fos,c-myc,K-ras和p53的表达。结果测序证明重组慢病毒高表达载体CYP3A4基因序列正确,荧光定量PCR检测CYP3A4高表达肝细胞株比正常肝细胞CYP3A4基因表达提高94倍。Western蛋白质印迹结果显示,CYP3A4高表达肝细胞株CYP3A4蛋白表达水平是正常肝细胞的2.36倍。CYP3A4高表达肝细胞bcl-2mRNA表达水平随三氯乙烯浓度增加呈下降趋势,与正常细胞相比,三氯乙烯0.25和0.5mmol·L-1使CYP3A4高表达肝细胞中的bcl-2mRNA明显升高(P<0.01);三氯乙烯0.5,1.0,2.0和4.0mmol·L-1处理使CYP3A4高表达肝细胞组的凋亡基因胱天蛋白酶3、胱天蛋白酶8和胱天蛋白酶9的mRNA表达水平明显升高(P<0.05);三氯乙烯0.5,1.0,2.0和4.0mmol·L-1处理的CYP3A4高表达肝细胞c-fos、c-myc和k-ras基因的表达显著升高(P<0.01),p53表达水平明显下降(P<0.01)。结论三氯乙烯对CYP3A4高表达肝细胞株中的凋亡基因和癌基因表达具有明显促进作用,说明CYP3A4是三氯乙烯在体内代谢的重要因素。

表没食子儿茶素-3-没食子酸酯对细胞色素P450酶活性的影响

目的研究表没食子儿茶素-3-没食子酸酯(EGCG)对人肝微粒体中细胞色素P450(CYP450)酶活性的影响。方法以未处理的肝微粒体作为阴性对照组,CYP450酶各亚型的特异性抑制剂作为阳性对照组,通过EGCG或特异性抑制剂与探针底物共同孵育,高效液相色谱法定量分析特异性底物的代谢产物,分析EGCG对CYP450酶各亚型活性的影响,并通过统计学分析拟合获得相应的动力学参数。结果与阴性对照组相比,EGCG显著抑制了CYP1A2酶和CYP3A4酶的活性,但抑制作用远小于阳性抑制剂的抑制作用。EGCG对CYP1A2酶和CYP3A4酶的抑制作用受EGCG浓度的影响,IC50值分别为8.69和14.07μmol/L。EGCG能够竞争性抑制CYP1A2酶的活性,而对CYP3A4酶为非竞争性抑制作用。此外,EGCG对CYP3A4酶的抑制作用具有时间依赖性,随着培养时间的延长,抑制作用逐渐增强。结论EGCG可显著抑制CYP1A2酶及CYP3A4酶的活性。因此,在EGCG的应用中应充分考虑可能出现的药物相互作用及潜在风险。

慢病毒介导的CYP3A11基因knock-down小鼠的建立

目的构建和筛选小鼠P4503A11基因miR RNAi慢病毒载体,建立CYP3A11基因knock-down小鼠。方法利用Ravi Sachidanandam's Lab的在线软件设计沉默小鼠P4503A11基因的miRNA所对应的shRNA序列,PCR扩增后克隆到PCI-GFP-MiR质粒中,其再与慢病毒载体FUW进行重组。将psPAX2和pMD2.G两个载体和FUW-GFP-MiR-shRNA重组慢病毒载体共转染293FT细胞,包装成病毒。用包装好的病毒液感染293FT细胞后,并利用GFP蛋白表达水平进行滴度测定。将上述重组慢病毒载体分别转染FVB/N小鼠肝细胞,转染48h后,检测P4503A11基因mRNA表达水平的变化。选取干扰效果最好的FUW-GFP-MiR-shRNA1重组慢病毒载体进行制备基因knock-down小鼠模型。用显微注射法将浓缩的shRNA1病毒液注射至FVB/N小鼠12细胞期胚胎透明带下。将注射后发育至22细胞期的胚胎移植至假孕受体母鼠,得F0代小鼠。在紫外光照射下利用滤光片观察GFP在小鼠活体内的表达水平。结果DNA测序结果显示3个重组慢病毒载体均与所设计的shRNA序列一致。检测的3个浓缩前慢病毒悬液的滴度均≥106TU/ml,经过高速离心对病毒进行浓缩和纯化,其滴度达到109TU/ml以上。转染FUW-GFP-MiR-shRNA1、2的2组肝细胞的P4503A11基因mRNA表达水平相对于空白对照组均显著下降(P<0.05),而转染阴性对照FUW-GFP-MiR-shRNA-NC的肝细胞P4503A11基因mRNA表达水平相对于空白对照组无明显改变。选用FUW-GFP-MiR-shRNA1慢病毒载体制备的F0代3A11基因knock-down小鼠,在紫外光照射下,阳性小鼠可见较强的荧光。结论构建并筛选出小鼠P4503A11基因有效的靶向miR RNAi慢病毒载体,并成功建立CYP3A11基因knock-down小鼠。

老年急性冠状动脉综合征患者CYP3A5基因多态性与临床疗效及预后的关系

目的探讨CYP3A5基因多态性与老年急性冠状动脉综合征(ACS)患者PCI术后替格瑞洛疗效及预后的关系。方法选择我院收治的492例老年ACS患者为研究对象,按随机对照表法分为常规治疗组和个体治疗组各246例。其中常规治疗组给予阿司匹林0.1 g/d联合氯吡格雷75 mg/d治疗;个体治疗组采用单核苷酸多态性基因分型技术进行CYP3A5基因型检测,分为突变基因型142例[AA基因型组(68例)、AG基因型组(74例)]和非突变基因型104例(GG基因型组),AA基因型组和AG基因型组给予拜阿司匹林0.1 g/d联合替格瑞洛90 mg 2次/d治疗,GG基因型组给予常规治疗组相同疗法,持续治疗12个月。采用血栓弹力图仪检测患者的血小板反应性,观察12个月内的ACS患者心源性死亡、再发心肌梗死及心绞痛等终点事件,并采用相对风险度分析CYP3A5基因突变与预后的相关性。结果与常规治疗组比较,个体治疗组总心血管事件发生率明显下降(11.79%vs 21.14%,P=0.005)。2组患者心源性死亡、再发心肌梗死、出血事件等比较无显著差异(P>0.05)。3组不同基因分型患者采取不同的个体化治疗方案,不良心血管事件发生率比较无显著差异(P>0.05);与个体治疗组比较,常规治疗组血小板抑制率明显下降[(48.84±4.71)%vs(60.52±4.27)%,P<0.05〛。随访12个月,CYP3A5基因多态性(AA+AG、GG)个体治疗组治疗后患者预后及不良心血管事件发生风险无显著相关(OR=0.116,95%CI:0.062~0.226,P=0.156;OR=0.158,95%CI:0.084~0.247,P=0.125)。结论CYP3A5基因多态性不影响PCI术后使用替格瑞洛治疗的老年ACS患者的疗效,不增出血风险,且与患者临床预后无明显关联。

Rice CYP703A3, a cytochrome P450 hydroxylase, is essential for development of anther cuticle and pollen exine

Anther cuticle and pollen exine act as protective envelopes for the male gametophyte or pollen grain, but the mechanism underlying the synthesis of these lipidic polymers remains unclear. Previously, a tapetum‐expressed CYP703A3, a putative cytochrome P450 fatty acid hydroxylase, was shown to be essential for male fertility in rice（Oryza sativa L.）. However,the biochemical and biological roles of CYP703A3 has not been characterized. Here, we observed that cyp703a3‐2 caused by one base insertion in CYP703A3 displays defective pollen exine and anther epicuticular layer, which differs from Arabidopsis cyp703a2 in which only defective pollen exine occurs. Consistently, chemical composition assay showed that levels of cutin monomers and wax components were dramatically reduced in cyp703a3‐2 anthers. Unlike the wide range of substrates of Arabidopsis CYP703A2, CYP703A3 functions as an in‐chain hydroxylase only for a specific substrate, lauric acid, preferably generating 7‐hydroxylated lauric acid. Moreover, chromatin immunoprecipitation and expression analyses revealed that the expression of CYP703A3 is directly regulated by Tapetum Degeneration Retardation, a known regulator of tapetum PCD and pollen exine formation. Collectively, our results suggest that CYP703A3 represents a conserved and diversified biochemical pathway for in‐chain hydroxylation of lauric acid required for the development of male organ in higher plants.

GSTT1,GSTM1 and CYP2E1 genetic polymorphisms in gastric cancer and chronic gastritis in a Brazilian population

AIM:To test the hypothesis that,in the Southeastern Brazilian population,the GSTT1,GSTM1 and CYP2E1 polymorphisms and putative risk factors are associated with an increased risk for gastric cancer. METHODS:We conducted a study on 100 cases of gastric cancer (GC),100 cases of chronic gastritis (CG),and 150 controls (C).Deletion of the GSTT1 and GSTM1 genes was assessed by multiplex PCR.CYP2E1/Pst1 genotyping was performed using a PCR-RFLP assay. RESULTS:No relationship between GSTT1/GSTM1 deletion and the c1/c2 genotype of CYP2E1 was observed among the three groups.However,a significant difference between CG and C was observed,due to a greater number of GSTT1/GSTM1 positive genotypes in the CG group.The GSTT1 null genotype occurred more frequently in Negroid subjects,and the GSTM1 null genotype in Caucasians,while the GSTM1 positive genotype was observed mainly in individuals with chronic gastritis infected with H pylori. CONCLUSION:Our findings indicate that there is no obvious relationship between the GSTT1,GSTM1 and CYP2E1 polymorphisms and gastric cancer.

GSTM1,GSTT1,GSTP1 and CYP1A1 genetic polymorphisms and susceptibility to esophageal cancer in a French population:Different pattern of squamous cell carcinoma and adenocarcinoma

AIM:To evaluate the association between CYP1A1 and GSTs genetic polymorphisms and susceptibility to esophageal squamous cell carcinoma(SCC)and esophageal adenocarcinoma(ADC)in a high risk area of northwest of France. METHODS:A case-control study was conducted to investigate the genetic polymorphisms of these enzymes (CYPIAI*2C and GSTP1 exon 7 Val alleles,GSTMI*2/*2 and GSTTl *2/*2 null genotypes).A total of 79 esophageal cancer cases and 130 controls were recruited. RESULTS:GSTMI*2/*2 and CYPIAI*IA/*2C genotype frequencies were higher among squamous cell carcinomas at a level dose to statistical significance(OR =1.83,95% CI 0.88-3.83,P=0.11;OR=3.03,95% CI 0.93-9.90,P=0.07, respectively).For GSTP1 polymorphism,no difference was found between controls and cases,whatever their histological status.Lower frequency of GSTT1 deletion was observed in ADC group compared to controls with a statistically significant difference(OR=13.31,95% CI 1.66-106.92,P<0.01). CONCLUSION:In SCC,our results are consistent with the strong association of this kind of tumour with tobacco exposure.In ADC,our results suggest 3 distinct hypotheses: (1)activation of exogenous procarcinogens,such as small halogenated compounds by GSTT1;(2)contribution of GSTT1 to the inflammatory response of esophageal mucosa,which is known to be a strong risk factor for ADC, possibly through leukotriene synthesis;(3)higher sensitivity to the inflammatory process associated with intracellular depletion of glutathione.

CYP1A1,CYP2E1 and EPHX1 polymorphisms in sporadic colorectal neoplasms

AIM To investigate the contribution of polymorphisms in the CYP1A1, CYP2E1 and EPHX1 genes on sporadic colorectal cancer(SCRC) risk. METHODS Six hundred forty-one individuals(227 patients with SCRC and 400 controls) were enrolled in the study. The variables analyzed were age, gender, tobacco and alcohol consumption, and clinical and histopathological tumor parameters. The CYP1A1 *2A, CYP1A1 *2C CYP2E1 *5B and CYP2E1 *6 polymorphisms were analyzed by polymerase chain reaction-restriction fragment length polymorphism(PCR-RFLP). The EPHX1 Tyr113 His, EPHX1 His139 Arg and CYP1A1 *2C polymorphisms were detected by real-time PCR. Chisquared test and binary logistic regression were used in the statistical analysis. Haplotype analysis was conducted using the Haploview program, version 2.05.RESULTS Age over 6 2 years was a risk factor for SCRC development(OR = 7.54, 95%CI: 4.94-11.50, P < 0.01). Male individuals were less susceptible to SCRC(OR = 0.55, 95%CI: 0.35-0.85, P < 0.01). The CYP2E1*5B polymorphism was associated with SCRC in the codominant(heterozygous genotype: OR = 2.66, 95%CI: 1.64-4.32, P < 0.01), dominant(OR = 2.82, 95%CI: 1.74-4.55, P < 0.01), overdominant(OR = 2.58, 95%CI: 1.59-4.19, P < 0.01), and log-additive models(OR = 2.84, 95%CI: 1.78-4.52, P < 0.01). The CYP2E1*6 polymorphism was associated with an increased SCRC risk in codominant(heterozygous genotype: OR = 2.81, 95%CI: 1.84-4.28, P < 0.01; homozygous polymorphic : OR = 7. 3 2, 9 5 % C I : 1.85-28.96, P < 0.01), dominant(OR = 2.97, 95%CI: 1.97-4.50, P < 0.01), recessive(OR = 5.26, 95%CI: 1.35-20.50, P = 0.016), overdominant(OR = 2.64, 95%CI: 1.74-4.01, P < 0.01), and log-additive models(OR = 2.78, 95%CI: 1.91-4.06, P < 0.01). The haplotype formed by the minor alleles of the CYP2E1*5B(C) and CYP2E1*6(A) polymorphisms was associated with SCRC(P = 0.002). However, the CYP1A1 *2A, CYP1A1 *2C, EPHX1 Tyr113 His and EPHX1 His139 Arg polymorphisms were not associated with SCRC.CONCLUSION In conclusion, the results demonstrated that CYP2E1*5B and CYP2E1*6 minor alleles play a role in the development of SCRC.

异烟肼和利福平联合用药对健康成人原代肝细胞CYP450同工酶1A2和3A4活性的影响

目的明确异烟肼和利福平联合用药对健康成人原代肝细胞CYP450同工酶1A2和3A4活性的影响。方法从健康成人肝脏或肝叶中分离出肝细胞,分为CYP450同工酶1A2和3A4两部分,各分为阴性对照组及药物处理组共15组,放入24孔细胞培养板内,每组6个复孔,原代培养3 d,阴性对照组加入等量的细胞培养液,各药物处理组对应加入临床血药峰浓度范围内的异烟肼(25μmol/L,50μmol/L)、利福平(12.5μmol/L,25μmol/L)或两药联用(CYP1A2:利福平12.5μmol/L加异烟肼50μmol/L,利福平25μmol/L加异烟肼50μmol/L;CYP3A4:利福平12.5μmol/L加异烟肼25μmol/L,利福平25μmol/L加异烟肼25μmol/L,利福平25μmol/L加异烟肼50μmol/L),孵育2 d,再加入CYP450同工酶1A2和3A4的相应底物(非那西丁和睾酮),反应终止后用高效液相仪测量代谢产物(对乙酰氨基酚与6β-羟基睾酮)的峰面积(单位:mAU.m in)代表1A2和3A4的活性。结果(1)单用25μmol/L和50μmol/L浓度异烟肼肝细胞CYP450同工酶1A2的活性分别是(3.33±0.65)、(3.03±0.38)mAU.m in,与阴性对照组的(5.23±0.31)mAU.m in比较差异均有统计学意义(P均<0.01);单用12.5μmol/L浓度利福平肝细胞CYP450同工酶1A2的活性为(6.07±0.55)mAU.m in,与阴性对照组比较差异有统计学意义(P<0.05),单用25μmol/L浓度利福平肝细胞CYP450同工酶1A2的活性为(4.93±0.57)mAU.m in,与阴性对照组比较差异无统计学意义(P>0.05);异烟肼和利福平2种浓度联合配伍,肝细胞CYP450同工酶3A4的活性分别是(3.27±0.96)、(3.97±0.25)mAU.m in,与阴性对照组比较差异均有统计学意义(P均<0.05)。(2)单用25μmol/L和50μmol/L浓度异烟肼肝细胞CYP450同工酶1A2的活性分别是(5.40±1.35)、(2.63±0.06)mAU.m in,与阴性对照组的(12.53±0.51)mAU.m in比较差异均有统计学意义(P均<0.01);单用12.5和25μmol/L浓度利福平肝细胞CYP450同工酶3A4的活性分别为(165.17±11.47)、(120.20±15.73)mAU.m in,与阴性对照组比较差异均有统计学意义(P均<0.01);异烟肼和利福平3种浓度联合配伍,肝细胞CYP450同工酶3A4的活性分别是(118.37±8.90)、(77.53±6.91)、(68.73±4.72)mAU.m in,与阴性对照组比较差异均有统计学意义(P均<0.01),但低于相应浓度单用利福平组(P<0.05或0.01)。结论临床血药峰浓度范围的异烟肼与利福平单用或联用对CYP450同工酶1A2活性影响未达到抑制或诱导水平。临床血药峰浓度范围的异烟肼抑制CYP450同工酶3A4的活性,利福平诱导CYP450同工酶3A4的活性,两药联合仍呈诱导作用。