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 ( CYP2 E1) is considered to play an important role in the metabolic activation of procarcinogens such as N-nitroscoamines and Iow molecular weight organic compounds. The purpose of this study is to determine whether CYP450 2Elpolymorphisms are associated with risk s 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 dsmographic characteristcs, diet intake, and alcohol and tobacco consumption of indivduals 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 indivduals in gastric cancer group(6.6%),whereas there was only one in the control group (1.1%).However, there was no statistically significan difference between the two groups (two-tailed Fisher′s exact test, P =0.066). Indivduals in gastric cancer group were more likely to carry genotype C1/C2 (odds ratio, OR = 1.50) and C2/C2(OR = 7.34) than indivduals in control group (X2 = 4.597, for trend P=0.032). The frequencies of genofypes with the C2allele ( C1/C2 and C2/C2 genotypes) were compared with those of genotypes without C2 allele ( C1/C1 genotype )among indivduals in gastric cancer group and control group according to the pattern of gastric cancer risk factors. The results show that indivduals 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 effct in the development of gastric cancer in Changle county, Fujian Province.

Hepatoprotective effects of S-adenosyl-L-methionine against alcohol-and cytochrome P450 2E1-induced liver injury

S-adenosyl-L-methionine (SAM) acts as a methyl donor for methylation reactions and participates in the synthesis of glutathione. SAM is also a key metabolite that regulates hepatocyte growth, differentiation and death. Hepatic SAM levels are decreased in animal models of alcohol liver injury and in patients with alcohol liver disease or viral cirrhosis. This review describes the protection by SAM against alcohol and cytochrome P450 2E1-dependent cytotoxicity both in vitro and in vivo and evaluates mechanisms for this protection.

Cytochrome P450 2E1 RsaI/PstI and DraI Polymorphisms Are Risk Factors for Lung Cancer in Mongolian and Han Population in Inner Mongolia

Objective： To explore the relationship between cytochrome P450 2E1 （CYP2E1） RsaI/PstI and DraI polymorphism and lung cancer susceptibility in Mongolian and Han population in Inner Mongolia of China. Methods： CYP2E1 RsaI/PstI and DraI polymorphisms were detected by polymerase chain reaction-restriction fragment length polymorphism in 64 lung cancer patients, 150 healthy Mongolian and 150 healthy Han individuals. The distribution of genotype and allele frequencies of CYP2E1 RsaI/PstI and DraI polymorphisms were studied. Results： The risk of lung cancer was increased in individuals with CYP2E1 （cl/cl） and CYP2E1 （DD） with OR values of 2.431 （95%CI=1.082-5.460） and 2.778 （95%CI=1.358-5.683） respectively （P0.05）. When CYP2E1 RsaI/PstI and DraI polymorphisms were combined, the risk of lung cancer was reduced in individuals with CYP2E1 （cl/c2＋c2/c2 and DD＋CC） with OR values of 0.233 （95%CI=0.088-0.615, P0.05）. In smokers, the susceptibility to lung cancer was higher in the individuals with CYP2E1 （c1/c1） and CYP2E1 （DD） than in the individuals with c2 and C allele （P0.05, OR=2.643 and 4.308 respectively）. There was no significant difference in distribution of CYP2E1 genotype frequency between healthy Mongolian, Han population and lung cancer patients, healthy controls in Inner Mongolia. Conclusion： CYP2E1 （c1/c1） and CYP2E1 （DD） are predisposing factors of lung cancer in population in Inner Mongolia. CYP2E1 （c2﹢C） co-mutation may decrease the risk of lung cancer. Smoking exerts synergetic effect with CYP2E1 （c1/c1） and CYP2E1 （DD） on the occurrence of lung cancer.

Cytochrome P450 family 17 subfamily A member 1 mutation causes severe pseudohermaphroditism: A case report

BACKGROUND 17α-Hydroxylase deficiency(17-OHD)is a rare form of congenital adrenal hyperplasia,characterized by hypertension,hypokalemia,and gonadal dysplasia.However,due to the lack of a comprehensive understanding of this disease,it is prone to misdiagnosis and missed diagnosis,and there is no complete cure.CASE SUMMARY We report a female patient with 17-OHD.The patient was admitted to the Department of Neurology of our hospital due to limb weakness.During treatment,it was found that the patient’s condition was difficult to correct except for hypokalemia,and her blood pressure was difficult to control with various antihypertensive drugs.She was then transferred to our department for further treatment.On physical examination,the patient's gonadal development was found to be abnormal,and chromosome analysis demonstrated karyotype 46,XY.Considering the possibility of 17-OHD,the cytochrome P450 family 17 subfamily A member 1(CYP17A1)test was performed to confirm the diagnosis.CONCLUSION The clinical manifestations of 17-OHD are complex.Hormone determination,imaging examination,chromosome determination and CYP17A1 gene test are helpful for early diagnosis.

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。

Influences of V5-epitope tag on the metabolic activation of AFB1 by human cytochrome P450 2A13

Objective： To explore the impact of V5-epitope tag inserted in the commercial pcDNA5/FRT/V5-His TOPO expression vector on the metabolic activation of AFB1 by human CYP2A13. Methods ： A C-terminal 6 × Histag was first introduced into CYP2A13 cDNA by PCR and subsequently transferred into the expressing vector pcDNA5/FRT. Another commercial pcDNA5/FRT/V5-His TOPO expression vector was used to develop the construct directly via PCR. Both of the constructs were then transfected into Flp-In CHO and allowed for the stable expression of CYP2A13. The mouse CYP2A5 and the vector alone were used as positive and negative control, respectively. The presence of CYP2A5 and CYP2A13 cDNA and their protein expression in the stable transfectant cells were deterrrfined by immunoblotting assay using a monoclonal antibody against 6 × Histag. The AFBl-induced cytotoxicity in these tranfected CHO cells were conducted by MTS assay and the IC50 of cell viability was used to compare the CYP enzyme metabolic activity in AFB1 metabolism among these cells. Results： In accordance with the Flp-In system working mechanism, all the transfectant cells presented same protein expression level. The CHO cells expressing CYP2A5 was more sensitive to AFB1 treatment than those cells expressing CYP2A13, there was about 30-fold ICs0 difference between the two cells （2.1 nmol/L vs 58 nmol/L）. Interestingly, CYP2A13 fused with V5-Histag had the lost of metabolic activity to AFB1 than that fused with Histag alone, the ICa, of the viability in CHO-2A13-His-V5 cells was about 20-fold less than CHO-2A13- His （〉 1 000 nmol/L vs 58 nmol/L）. However, there was no change between CYP2A5 fused with V5-Histag and Histag alone （2.4 nmol/L vs 2.1 nmol/L）. Conclusion： The results demonstrate that CYP2A13 fused with V5-epitope has a significant impact on its metabolic activation to AFB1, which indicated that it should be careful to select a new expressing vector for evaluating the enzyme activity in carcinogen metabolism.

<i>In vivo</i>effects of genistein, herbimycin a and geldanamycin on rat hepatic cytochrome P4501A

Cytochrome P4501A (the CYP1A1 and CYP1A2 enzymes) are regulated through the aryl hydrocarbon receptor (AhR)-dependent signal transduction pathway and are generally known as enzymes which metabolize anthropogenic xenobiotics such as dioxin to carcinogenic and mutagenic compounds. However, recently the facts of CYP1A activation under physiological conditions or under action of non-dioxin-like compounds appear. In the present study we show that genistein, herbimycin A and geldanamycin (the protein-tyrosine kinase inhibitors) affect in vivo to CYP1A1 activity, the CYP1A1 mRNA level and the CYP1A1 protein level. These data provide insight into the role of protein kinases in CYP1A regulation may facilitate the understanding of CYP1A regulation.

河南汉族人群细胞色素P-450 1A1与肺癌易感性的关系

目的:探讨CYP1A1基因多态与支气管肺癌癌变关系。方法:采用病例-对照设计和PCR-RFLP方法,检测肺癌组103例和对照组138例CYP1A1基因多态,以logistic回归模型计算比数比(odds ratios,OR)及95%可信区间(confidential intervals,CI)。结果:CYP1A1m1突变型等位基因频率在对照组和肺癌组分别为27.6%和42.7%。logistic回归分析表明,CYP1A1(w1/m1)杂合型(B型)和(m1/m1)纯合突变型(C型)患肺癌的危险度分别升高3.19和2.61倍,差异显著。结论:CYP1A m1突变型等位基因是患肺癌的危险因素。

Functionalized selenium nanoparticles ameliorated acetaminophen-induced hepatotoxicity through synergistically triggering PKCδ/Nrf2 signaling pathway and inhibiting CYP 2E1

Selenium nanoparticles(SeNPs)have been demonstrated potential for use in diseases associated with oxidative stress.Functionalized SeNPs with lower toxicity and higher biocompatibility could bring better therapeutic activity and clinical application value.Herein,this work was conducted to investigate the protective effect of Pleurotus tuber-regium polysaccharide-protein complex funtionnalized SeNPs(PTR-SeNPs)against acetaminophen(APAP)-induced oxidative injure in HepG2 cells and C57BL/6J mouse liver.Further elucidation of the underlying molecular mechanism,in particular their modulation of Nrf2 signaling pathway was also performed.The results showed that PTR-SeNPs could significantly ameliorate APAP-induced oxidative injury as evidenced by a range of biochemical analysis,histopathological examination and immunoblotting study.PTR-SeNPs could hosphorylate and activate PKCδ,depress Keap1,and increase nuclear accumulation of Nrf2,resulting in upregulation of GCLC,GCLM,HO-1 and NQO-1 expression.Besides,PTR-SeNPs suppressed the biotransformation of APAP to generate intracellular ROS through CYP 2E1 inhibition,restoring the mitochondrial morphology.Furthermore,the protective effect of PTR-SeNPs against APAP induced hepatotoxicity was weakened as Nrf2 was depleted in vivo,indicating the pivotal role of Nrf2 signaling pathway in PTR-SeNPs mediated hepatoprotective efficacy.Being a potential hepatic protectant,PTR-SeNPs could serve as a new source of selenium supplement for health-promoting and biomedical applications.

检测细胞色素P-450基因族中CYP1A1基因表达的一个简捷方法(英文)

NMR1系雄性小鼠被用来研究肺微粒体细胞色素P450家族中一个同功基因CYP1A1在香烟烟雾的诱导下表达.双轮回‘聚合酶链式反应’(PCR)和‘反向转录酶-聚合酶链式反应’(RT-PCR)被用来检测基因CYP1A1的转录水平.代表CYP1A1蛋白活性的7-乙氧基试卤灵-0-去乙基酶(EROD)的活性被用来检测基因CYP1A1的表达.双轮回‘聚合酶链式反应’(PCR)和‘反向转录酶-聚合酶链式反应’(RT-PCR)被用来检测基因CYP1A1的转录水平.测试结果表明在吸入香烟烟雾的情况下,小鼠肺微粒体EROD的活性和基因CYP1A1的转录水平是同步增加的.这个结果不同于以前在同样实验条件的一个自相矛盾的结果,即在CYP1A1蛋白增加时,基因CYP1A1的转录水平却是下降或不变.这说明本文所使用的方法可能要优于以前的实验方法.

尿道癌相关基因1通过微小RNA-513a-3p/细胞色素P_(450)1B1生物学轴促进人胃癌细胞增殖和迁移的机制研究

目的研究长链非编码RNA(lncRNA)尿路上皮癌胚抗原1(UCA1)在人胃癌细胞中的表达,并探讨UCA1通过微小RNA-513a-3p(miR-513a-3p)/细胞色素P_(450)1B1(CYP1B1)生物学轴对胃癌细胞增殖和迁移的影响及机制。方法分别向人胃癌细胞中转入UCA1小干扰RNA(siRNA)、miR-513a-3p模拟物和miR-513a-3p抑制剂以抑制UCA1、上调miR-513a-3p和抑制miR-513a-3p表达。通过定量PCR检测不同细胞UCA1、miR-513a-3p和CYP1B1 mRNA的表达,CCK8试剂盒检测细胞增殖,Transwell小室检测细胞迁移。结果与GES-1细胞相比,UCA1在人胃癌细胞HGC-27、SNU-5、AGS、SGC-7901中表达均升高(t=11.106,P<0.001;t=10.872,P<0.001;t=12.134,P<0.001;t=16.178,P<0.001),细胞增殖活性(t=7.252,P<0.001;t=8.964,P<0.001;t=8.666,P=0.003;t=8.697,P<0.001)和细胞迁移能力(t=4.040,P=0.010;t=7.079,P<0.001;t=6.833,P=0.003;t=7.527,P<0.001)均升高。双荧素酶基因报告实验显示miR-513a-3p与UCA1和CYP1B1靶向结合。与NC siRNA组相比,UCA1 siRNA显著下调UCA1和上调miR-513a-3p在SGC-7901细胞中的表达(t=7.895,P<0.001;t=12.911,P<0.001);miR-513a-3p表达上调显著抑制SGC-7901细胞中UCA1和CYP1B1 mRNA表达(t=7.224,P<0.001;t=5.645,P=0.002),而抑制miR-513a-3p则显著上调SGC-7901细胞中UCA1和CYP1B1 mRNA表达(t=9.628,P<0.001;t=11.665,P<0.001)。与单独UCA1敲低的SGC-7901细胞相比,UCA1和miR-513a-3p共同敲低的SGC-7901细胞CYP1B1 mRNA表达、细胞增殖活性和细胞迁移能力均升高(t=3.695,P=0.014;t=4.198,P=0.009;t=3.602,P=0.016)。结论UCA1通过miR-513a-3p/CYP1B1生物学轴促进人胃癌细胞的增殖和迁移。

细胞色素P4501A1基因多态性与喉癌遗传易感性的研究

目的 探讨细胞色素P45 0 1A1(cytochromep45 0 1A1,CYP1A1)MspI多态性与喉癌易感性之间的关系。方法 以病例 对照研究 ,采用聚合酶链反应 限制性片段长度多态性分析 (polymerasechainreactionrestrictionfragmentlengthpolymorphism ,PCR RFLP)方法检测 6 2例喉鳞状细胞癌和 5 6例健康对照CYP1A1的基因型 ,并按吸烟指数 (smokingindex ,SI,吸烟支数 /d×吸烟年数 )的不同分析患喉癌风险。结果 CYP1A1MspI分为野生型A、突变杂合型B和突变纯合型C的 3种基因型。杂合型B和突变纯合型C在病例组分别占 5 8 1%和 14 5 % ,对照组分别占 39 3%和 7 1% ,两两比较 ,病例组杂合型B、纯合型C显著高于对照组 ,P <0 0 5 ,比值比率 (oddsration ,OR)分别为 2 89(95 %可信限1 31～ 6 37)和 3 97(95 %可信限 1 10～ 14 2 8)。在低吸烟量组 (SI≤ 40 0 )和高吸烟剂量组 (SI >40 0 )中 ,纯合型C的OR值分别为 4 5 (95 %可信限 0 6 4～ 31 6 1)和 9(95 %可信限 1 6 0～ 5 0 74)。结论 CYP1A1MspI多态性与吸烟协同在喉癌的发生、发展中可能起重要作用。突变纯合型个体患喉癌风险增加 ,吸烟时间越长 ,量越大 。

细胞色素P4502E1(CYP2E1)与胃癌遗传易感性

为探讨细胞色素P4502E1(CYP2E1)基因变化与胃癌易感的关系,采用病例—对照分子流行病学研究方法和多聚酶链反应技术—限制性片段长度多态性(PCR—RFLP),对142例胃癌患者和167例正常对照者CYP2E1基因RsaⅠ酶切位点进行多态性分析。结果显示胃癌患者和正常对照人群在基因型和等位基因频率上均无显著的统计学差异;我国人群CYP2E1 RsaⅠ酶切位点多态性的分布频率与日本人群相近,与欧美人群差异较大。

稳定表达人细胞色素P4501A2的HepG2细胞的建立及其代谢效应

目的 :建立稳定表达人细胞的色素 P4 5 0 1A2 (CYP1A2 )的 Hep G2细胞。方法 :将所克隆的野生型CYP1A2 c DNA从重组质粒 p GEM- CYP1A2中用 Kpn / Bam H 双酶切 ,并亚克隆到哺乳动物细胞表达载体p REP9中。再将重组质粒转化感受态大肠杆菌 Top10 ,用氨苄青霉素抗性筛选和限制酶谱鉴定。改良的磷酸钙介导的细胞转染法将重组质粒 p REP9- CYP1A2转染肝癌细胞 Hep G2 ,用 RT- PCR技术对转基因细胞的 CYP1A2m RNA表达作了分析 ,并用 MTT法比较转基因细胞对黄曲霉素 B1(AFB1)细胞毒敏感试验。结果 :与 Hep G2细胞相比 ,Hep G2 - CYP1A2转基因细胞表达 CYP1A2 m RNA,能增强 AFB1的细胞毒作用。结论 :建立了稳定表达CYP1A2的转基因细胞系 ,可用于由 CYP1A2参与的毒理学与药物代谢研究。

CYP1A1 MspI多态性与子宫内膜癌易感性的病例对照研究

自20世纪60年代以来，上海市区子宫内膜癌发病率逐年上升，且发病年龄有年轻化的趋势。子宫内膜癌的发病机制目前还不十分明确，多数流行病学研究显示子宫内膜癌的危险因素都与雌激素有关，雌激素水平升高导致的内膜增生及DNA损伤被认为是子宫内膜癌发生的主要机制。

CYP2E1基因多态和血清硒水平与肺癌关系的研究

目的：探讨CYP2E1基因RsaⅠ多态性单独作用和血清硒水平联合作用时与肺癌危险性的关系。方法：采用成组病例一对照研究方法，选择广州地区原发性肺癌患者58例，对照62例，制定统一调查表进行调查，用PCR检测CYP2E1基因多态性，用GHAFS测定血清硒。结果：CYP2E13种基因型在病例组与对照组的总体分布无统计学意义（X^2=1.578，P=0．454），CYP2E1多态性单独作用时与肺癌危险性关系无统计学意义（P〉0．05）；血清硒水平低（〈0．109mg／L）联合CYP2E1 C1C1基因型时OR为9．86（95％CI=1．13～85．99）。结论：CYP2E1基因单独作用与广州地区肺癌关系不明显，但血清硒水平低与CYP2E1 C1C1基因型之间存在协同作用，使肺癌发生的危险性显著增加。

CYP2C9、VKORC1基因多态性与华法林个体化用药研究进展

尽管具有治疗指数狭窄和出血并发症频繁的弊病,华法林仍是临床上应用非常广泛的口服抗凝血药物。不同患者对华法林的反应差异很大,在达到相同治疗效果的情况下,不同个体的用药剂量可能相差20倍之多。华法林的治疗剂量受多种因素影响,包括基因多态性、体重指数、年龄等及其他药物因素等,这就要求临床医师在应用华法林时需注重个体化用药及选择最优治疗方案。多种基因可影响华法林的药物代谢,其中细胞色素P450 2C9(CYP2C9)及维生素K环氧化物还原酶复合体1(VKORC1)基因多态性是目前研究的重点。本文将综述以上两个基因的基因多态性及其与华法林个体化用药相关性的研究进展。

Use of cafeine as a probe for rapid determination of cytochrome P-450 CYP1A2 activity in humans

目的：建立快速测定细胞色素Ｐ４５０ＣＹＰ１Ａ２酶活性的高压液相色谱方法．方法：取３００μＬ血浆样品，用β羟乙基茶碱作内标，经５ｍＬ氯仿／异丙醇（９∶１）萃取处理后，用００５％的乙酸、乙腈和甲醇作为基本流动相，采用梯度洗脱程序在ＯＤＳ柱上分离待测组分，紫外检测波长２８２ｎｍ．结果：无内源性物质干扰测定．次黄嘌呤、内标和咖啡因快速基线分离，三者的保留时间均小于１３分钟．次黄嘌呤和咖啡因的检测下限均为０１μｍｏｌ·Ｌ－１，线性范围分别为１－１００μｍｏｌ·Ｌ－１和１－２００μｍｏｌ·Ｌ－１，相关系数分别为０９９９９和０９９８７，变异系数分别小于６％和１０％．两者的平均相对回收率为９６％－１０８％．结论：本方法快速、灵敏，可用于人群ＣＹＰ１Ａ２酶活性研究．

CYP2C9及VKORC1基因多态性对心脏瓣膜置换术后华法林个体剂量差异的研究

目的研究湖北地区汉族人细胞色素P450酶2C9(CYP2C9)基因和维生素K环氧化物还原酶复合体1(VKORC1)基因多态性分布特点及其对华法林稳态剂量的影响。方法收集2012年3—8月湖北地区汉族临床使用华法林的患者108例作为华法林组,选择同期健康受试者85名为对照组。采用聚合酶链反应-限制性内切酶片段长度多态性(PCR-RFLP)技术检测CYP2C9和VKORC1基因型,并比较不同基因型华法林稳态剂量。结果两组基因型频率和等位基因频率分布比较差异无统计学意义(P>0.05)。华法林组中CYP2C9基因*1/*3型较*1/*1型华法林稳态剂量小,VKORC1基因AA型较GA型华法林稳态剂量小(P<0.05,P<0.01)。除了检测的3个多态位点,还发现了50多个变异位点。结论在湖北地区汉族人群中,存在CYP2C9和VKORC1基因多态性,且不同基因型患者间华法林稳态剂量存在差异,华法林基因相关变异位点需要进一步证实。

丹参酮对大鼠细胞色素P-450酶系和谷胱甘肽转移酶的作用

目的探讨丹参有效成分丹参酮 (Tan)对大鼠肝、肾组织内的细胞色素P 450酶 (cytochromeP 450,CYP)系和谷胱甘肽转移酶(GT)的影响。方法给予SD雄性大鼠丹参酮 (100mg·kg-1 )灌胃,每日 1次,连续10天后,选用CYP1A1、1A2、2B1、2E1及 3A特异性代谢底物,检测它们在肝和肾微粒体中的活性,同时检测肝、肾微粒体中的GT水平变化。结果实验表明,丹参酮可诱导肝微粒体内的CYP1A1、CYP1A2和CYP2B1活性显著升高(均P<0. 01),同时显著抑制CYP2E1的活性 (P<0. 01),也可诱导肝微粒体中GT的活性升高 (P<0.05)。结论丹参酮对CYP亚型的不同调节作用可能会影响与其合用药物在体内的代谢消除,丹参酮对GT的影响也具有一定的临床意义。