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1.
二氢叶酸还原酶是核酸代谢中的关键酶之一,是肿瘤化疗药物的主要靶酶。随着人们对其在基因水平研究的逐渐深入,发现氨甲蝶呤的靶酶二氢叶酸还原酶是引起耐药的主要原因。本文就二氢叶酸还原酶结构、功能及其与肿瘤耐药关系作一综述,并探讨其在临床的应用前景和意义。  相似文献   

2.
李玲  王明钰  徐海 《微生物学报》2021,61(12):4097-4105
[目的] 分析新型甲氧苄啶获得性耐药蛋白DfrB7的生化性质,探究其与B家族代表性的二氢叶酸还原酶(DHFR)对甲氧苄啶获得性耐药的生化基础。[方法] 构建系统进化树分析B家族DHFRs与新型DfrB7的进化关系。将dfr基因分别构建到pACYC184和pET15b(+)载体并转化到相应大肠杆菌中。使用微量肉汤稀释法确定克隆菌株对甲氧苄啶的耐药性。测定DHFRs使用NADPH作为质子供体催化二氢叶酸还原的酶活反应参数。通过等温滴定量热法测定甲氧苄啶的解离常数。[结果] 克隆到大肠杆菌中的新型dfrB7基因表现出对甲氧苄啶的高耐药表型。系统进化树确定了dfrB7编码B家族的DHFRs。检测并比较DfrB7和代表性DHFRs的酶活性质、抑制剂的亲和力,与染色体上DHFR相比,DfrB7与DfrB1均表现出显著降低的催化活性,通过生化实验证实B家族二氢叶酸还原酶对甲氧苄啶结合力极差。[结论] 新型dfrB7基因编码的DfrB7具有B家族二氢叶酸还原酶的普遍特征。B家族二氢叶酸还原酶赋予宿主菌对甲氧苄啶的获得性耐药与该酶对甲氧苄啶的低亲和力有关。  相似文献   

3.
在L615细胞株的细胞中发现有双微体(DM)。同样,这种细胞株的细胞中也有均质染色质区(HSR)的染色体。这条染色体为中度长短,HSR位于这条染色体的中部靠近顶端着丝点处。DM和HSR都是二氢叶酸还原酶(DHFR)基因的顺序,它们是DHFR基因的扩增。由于DHFR基因的扩增,细胞超量产生二氢叶酸还原酶,所以L615细胞对叶酸的同系物药物——氨甲喋呤(MTX)是抗性的。  相似文献   

4.
报道了带有His-tag的仓鼠二氢叶酸还原酶基因的克隆和在DB序列增强下T7启动子调控该基因在大肠杆菌中的可溶性高效表达,SDS-PAGE分析表明,带有His-tag的仓鼠二氢叶酸还原酶的含量可占大肠杆菌细胞总蛋白质含量的46%.该酶的纯化可用常规的金属络合树脂一步纯化至SDS-PAGE一条带,经凝血酶切去His-tag的仓鼠二氢叶酸还原酶与用等电聚焦法获得的无His-tag的酶有相同的酶活性.  相似文献   

5.
941449重组CHO细胞在其细胞周期中表达外源基因(β-半乳糖苷酶)[英]/Gu,M.B.…∥Biotechnol.Bioeng.-1993,42(9).-1113~1123[译自DBA,1993,12(25),93-14684] 用含二氢叶酸-还原酶基因(dhfr)和编码细菌β-半乳糖苷酶的LacZ基因的表达载体转染CHOβ-G72-16细胞,研究了单个该细胞中的外源蛋白  相似文献   

6.
用蛋白质内源荧光、疏水荧光探针TNS及蛋白酶K限制性酶解等方法研究了二氢叶酸还原酶在盐酸胍变性过程中的构象变化及动力学,并与活力变化进行了比较.TNS可以监测到与激活同步的构象变化;盐酸胍浓度大于0.75mol/L时,二氢叶酸还原酶被蛋白酶K水解速度增大;当盐酸胍浓度大于1.2mol/L时,才能监测到酶分子整体构象的变化.以上结果表明二氢叶酸还原酶在盐酸胍溶液中的变性并不符合标准的二态模型,而是先经历构象逐步松散的序变过程,然后发生协同的构象伸展.二氢叶酸还原酶在低浓度盐酸胍溶液中的激活是由于酶活性部位构象的微小变化引起的.酶活性部位构象的变化虽然降低了酶与废物的结合能力,但加快了酶促反应限速步骤,即底物解离速度而使酶活力升高.  相似文献   

7.
鸡肝二氢叶酸还原酶(DHFR)平衡态的去折叠曲线符合二态模型,但在4.0mol/L脲中的去折叠动力学为两相。该酶的ArrehiusPlot有一个拐点,但在低浓度变性剂存在下,拐点消失。用二氢叶酸还原酶的天然状态存在两种构象可以很好地解释上述现象。二氢叶酸还原酶去折叠过程中没有稳定存在的中间体,动力学过程中的两相可能是两种天然构象态的去折叠速度常数不同造成的。ArrehiusPlot的拐点是由于在不同的温度条件下,两种天然构象的含量不同造成的,低浓度变性剂对两种构象的影响不同,使拐点消失。KCl可以改变两种构象的平衡  相似文献   

8.
昆虫抗药性中的酯酶基因扩增研究进展   总被引:5,自引:1,他引:4  
唐振华 《昆虫知识》1993,30(1):53-56
<正> 基因扩增是基因组数量上呈现的不固定性,是通过改变基因组中某些基因的数量而使其产物增加的过程。 自Alt等发现哺乳动物培养细胞对药物氨甲蝶呤(methotrexate,MTX)产生抗性是由于二氢叶酸还原酶(dihydrofolate reductase,DHFR)基因扩增所致以后,在各种动物的抗  相似文献   

9.
目的:构建携带人二氢叶酸还原酶(DHFR)基因的慢病毒表达载体pWPI。方法:采用PCR方法扩增二氢叶酸还原酶cDNA全长,与EZ-T克隆载体连接,HindIII及BamHI-HF限制性内切酶双酶切回收的PCR片段并补平其缺口。慢病毒系统载体使用pWPI系统,采用PmeI酶切载体后回收片段,将其磷酸化,T4酶连接载体与目的基因。表达载体鉴定均采用核苷酸序列测定,重组质粒采用脂质体转染293T包装细胞后获得包装的病毒颗粒。结果:成功扩增二氢叶酸还原酶全长并连接入pWPI载体构建成重组表达载体DHFR-pWPI,重组质粒测序结果显与DHFR基因的同源性达100%,按标准生产程序转染293T后有DHFR基因的表达。结论:成功采用慢病毒载体系统构建了二氢叶酸还原酶重组慢病毒转基因,为探讨DHFR在肿瘤多药耐药过程中的分子机理奠定基础。  相似文献   

10.
人白细胞介素6(IL-6)是一种关键的多功能的细胞因子,它对造血、免疫和急性期应答起重要作用。重组IL-6在辐射损伤,血小板减少、肝损伤、肿瘤及艾滋病的研究与治疗中具有重要意义和潜在的应用前景。本研究通过引物设计、转译优化及DNA体外重组等技术构建了pSV-IL-6重组质粒,在大肠杆菌中大量扩增、纯化后,利用磷酸钙共沉淀法转染中国仓鼠卵巢细胞二氢叶酸还原酶缺陷株(CHO-dhfr~ ),经选择培养基培养2周后,挑出CHO-dhfr~ 细胞克隆,并用逐渐提  相似文献   

11.
Previous research has shown that a urinary pheromone of female mice acts via the vomeronasal organ of the accessory olfactory system to elicit rapid release of luteinizing hormone (LH) in conspecific males. Several experiments were conducted to examine the importance of sexual experience for gonadotropin responses in male mice to female urine, male urine, saline, or mixtures of these stimuli. Both sexually naive and sexually experienced male mice had significantly higher plasma LH levels after presentations of female urine than after presentations of male urine. However, sexual experience appeared to increase the reliability of the short-latency gonadotropin response to female urine relative to a sexually neutral component of urine such as sodium chloride, and male urine appeared to suppress spontaneous LH secretion episodes in both naive and sexually experienced males. Subsequent experiments with sexually experienced subjects demonstrated that male mouse urine is a powerful suppressant of LH release in other males. Specifically, female mouse urine mixed with male urine failed to elicit LH responses in male subjects, whereas female urine mixed with saline was highly effective. Urine obtained from castrated male donors was as potent as urine from intact males in suppressing the gonadotropin response to female urine. The suppressive activity in male mouse urine thus does not appear to be critically dependent on gonadal hormones. The existence of a potent stimulatory pheromone in female urine and a potent suppressive pheromone in male urine makes male mice an excellent model system for studying the neural regulation of LH secretion.  相似文献   

12.
The sexual development of female mice is accelerated by exposure to an adult male or to male urine. The component of the urine responsible for this effect is androgen-dependent, heat labile, nondialysable, precipitatable with ammonium sulphate, and is not extractable in ether. These results indicate that the pheromone causing accelerated sexual development is associated with a protein component of male urine. Tests of the active fraction after digestion with proteolytic enzymes suggest that the pheromone may be a portion of a protein or a substance bound to a protein.  相似文献   

13.
The simultaneous determination of trimethoprim, sulphamethoxazole and N4-acetyl-sulphamethoxazole in serum and urine by high-performance liquid chromatography using sulphafurazole as internal standard is described. The separation was achieved on a reversed-phase column employing acetic acid—methanol as the mobile phase with spectrophotometric detection at 230 nm. Precise simultaneous quantitative analysis of the relative components has been achieved at levels of 0.1 μg/ml for trimethoprim and 1.0 μg/ml for both sulphamethoxazole and its N4-acetyl metabolize using 1 ml of serum or urine.  相似文献   

14.
Urine concentrates from 17 cigarette-smoking baboons and 12 sham puffers were analyzed for mutagenic activity in S. typhimurium tester strain TA1538. Both the proportion of animals exhibiting measurable mutagenic activity in urine and the mean level of mutagenic activity present were significantly greater in cigarette smoking baboons (P less than 0.05). Mutagenic activity in the urine of male and female cigarette-smoking baboons was not significantly different. Age and smoking history did not, but mean blood carboxyhemoglobin did, correlate with mutagenic activity of the urine concentrate from individual animals. Fractionation of the urine concentrates on silicic acid separated the concentrate into fractions that were more active in TA100 and others that were more active in TA1538. Further fractionation was accomplished by HPLC.  相似文献   

15.
DAVITIYANANDA, DANIS and FOLKE RASMUSSEN: Mammary and renal excretion of sulphadoxine and trimethoprim in cows. Acta vet. scand. 1974, 15, 340–355. — In 21 experiments on 5 healthy, nonpregnant cows are sulphadoxine and trimethoprim infused intravenously for maintenance of constant levels of the drugs through the experimental periods. The experiments show that both sulphadoxine and trimethoprim are bound to the proteins in blood plasma and milk. Further it is demonstrated that sulphadoxine (an acid) is excreted into milk in concentrations lower than in blood plasma while trimethoprim (a base) is excreted into milk in concentrations higher than in blood plasma. Both results are consistent with the theory that drugs are excreted through the mammary gland by passive diffusion. Glomerular filtration and back-diffusion are both involved in the renal handling of sulphadoxine and trimethoprim. For trimethoprim active tubular secretion is also demonstrated. Both the mammary and renal handling of sulphadoxine as well as trimethoprim are influenced by the pH of milk and urine, respectively. The experiments underline that it is the unionized, non-protein-bound fraction of the drugs which diffuses through biological membranes. sulphadoxine; trimethoprim; mammary excretion; renal excretion; cow.  相似文献   

16.
This paper describes the identification of a new bile alcohol possessing the 5 alpha-cholestane structure that was found in the urine of patients with cerebrotendinous xanthomatosis. The urine samples were extracted with reversed-phase resin, treated with beta-glucuronidase, and separated on silica gel and reversed-phase column chromatography. The new bile alcohol isolated was the second component of the urinary bile alcohols and was identified as (23S)-5 alpha-cholestane-3 alpha,7 alpha,12 alpha,23,25-pentol by means of gas-liquid chromatography/mass spectrometry and nuclear magnetic resonance spectroscopic studies.  相似文献   

17.
Purification and characterization of rat urinary esterase A1   总被引:1,自引:0,他引:1  
An enzyme, esterase A1, which hydrolyzes tosyl-arginine methyl ester (Tos-Arg-OMe) was separated from esterase A2 and kallikrein of male rat urine and purified by a procedure involving ammonium sulfate fractionation, ion exchange chromatography, hydrophobic chromatography and gel filtration. The resulting preparation was apparently homogeneous, as assessed by polyacrylamide gel electrophoresis. The molecular weight of the preparation was estimated to be 27,000 by SDS-polyacrylamide gel electrophoresis and 30,000 by gel filtration. The enzyme was more specific for arginine methyl esters than for lysine methyl esters. The optimum pH determined with Tos-Arg-OMe as a substrate was 8.0 and the Km was 11.8 mM. The Tos-Arg-OMe esterolytic activity of esterase A1 was inhibited by soybean trypsin inhibitor, but not by aprotinin. In immunodiffusion analysis, the antiserum to esterase A1 formed immunoprecipitin arcs with this enzyme and the urine collected from rat bladder, but not with esterase A2, kallikrein, plasma and the urine collected from ureters. These results indicate that rat urinary esterase A1 differs from esterase A2 and kallikrein. The esterase A1 appears to be produced by accessory sex glands and excreted via the spermiduct into the urine.  相似文献   

18.
The absolute configuration of 2-sec-butyl-4,5-dihydrothiazole (DHT) in urine of adult male mice was determined through chiral trifluoroacetyl derivative capillary chromatography by comparing the retention time with synthetic standards. (S)-DHT was extracted from fresh urine, while neither (R)-DHT nor the racemization of (S)-DHT were detected. We can conclude that DHT in urine possesses the S configuration, although we cannot exclude a minor component in the R configuration. (S)-DHT was then characterized for binding to the complex of major urinary proteins of male mouse urine (MUP) and for a behavioral response, the competitive scent marking behavior (countermarking). The binding constant of (S)-DHT to MUP (determined by competitive displacement) was 8.2 +/- 0.6 microM (mean +/- SD) and was 10.5 +/- 0.6 microM for R-DHT, thus excluding a relevant difference in binding. (S)-DHT modified countermarking in a peculiar way. Male mice were slow in countermarking urinary spots streaked 2 days earlier and on top of which (S)-DHT was added shortly before the test. This response was not seen when adding (S)-DHT to freshly streaked urinary spots or to clean paper. Unlike (S)-DHT, (R)-DHT prompted countermarking rather than delaying it. We can further conclude that (S)-DHT in male mouse urine is an aversive chemosignal for countermarking.  相似文献   

19.
For women with recurrent urinary tract infections (rUTI), the contribution of antibiotic use versus patient-related factors in determining the presence of antimicrobial resistance in faecal and urinary Escherichia coli, obtained from the same patient population, has not been assessed yet. Within the context of the ‘Non-antibiotic prophylaxis for recurrent urinary tract infections’ (NAPRUTI) study, the present study assessed determinants of antimicrobial resistance in E. coli isolated from urinary and faecal samples of women with rUTIs collected at baseline. Potential determinants of resistance were retrieved from self-administered questionnaires. From 434 asymptomatic women, 433 urinary and 424 faecal samples were obtained. E. coli was isolated from 146 (34%) urinary samples and from 336 (79%) faecal samples, and subsequently tested for antimicrobial susceptibility. Multivariable analysis showed trimethoprim/sulfamethoxazole (SXT) use three months prior to inclusion to be associated with urine E. coli resistance to amoxicillin (OR 3.6, 95% confidence interval: 1.3–9.9), amoxicillin-clavulanic acid (OR 4.4, 1.5–13.3), trimethoprim (OR 3.9, 1.4–10.5) and SXT (OR 3.2, 1.2–8.5), and with faecal E. coli resistance to trimethoprim (OR 2.0, 1.0–3.7). The number of UTIs in the preceding year was correlated with urine E. coli resistance to amoxicillin-clavulanic acid (OR 1.11, 1.01–1.22), trimethoprim (OR 1.13, 1.03–1.23) and SXT (OR 1.10, 1.01–1.19). Age was predictive for faecal E. coli resistance to amoxicillin (OR 1.02, 1.00–1.03), norfloxacin and ciprofloxacin (both OR 1.03, 1.01–1.06). In conclusion, in women with rUTI different determinants were found for urinary and faecal E. coli resistance. Previous antibiotic use and UTI history were associated with urine E. coli resistance and age was a predictor of faecal E. coli resistance. These associations could best be explained by cumulative antibiotic use.  相似文献   

20.
Establishment of a near-standard two-dimensional human urine proteomic map   总被引:9,自引:0,他引:9  
Oh J  Pyo JH  Jo EH  Hwang SI  Kang SC  Jung JH  Park EK  Kim SY  Choi JY  Lim J 《Proteomics》2004,4(11):3485-3497
A proteomic map for human urine on two-dimensional (2-D) gels has been developed. Initial studies demonstrated that the urine proteins prepared by conventional methods showed interference and poor reproducibility in 2-D electrophoresis (2-DE). To address this issue, urine samples were dialyzed to remove any interfering molecules. The dialysis of urine proteins and the concentration by lyophilization without fractionation significantly improved the reproducibility and resolution and likely represents the total urine proteins on a 2-D gel. In addition, removing albumin from urine using Affi-Gel Blue helped to identify the low-abundant proteins. Using the developed method, we prepared proteins from urine collected from healthy females and males. The large inter- and intra-subject variation in protein profiles on 2-D gels made it difficult to establish a normal human urine proteomic 2-D map. To resolve this problem, urinary proteins were prepared from the pooled urine collected from 20 healthy females and males, respectively. The established male and female urine proteomes separated on 2-D gels were almost identical except for some potential sex-dependent protein spots. We have annotated 113 different proteins on the 2-D gel by peptide mass fingerprinting (PMF). We propose that the established total urine proteome can be used for 2-DE analysis, liquid chromatography-tandem mass spectrometry (LC-MS/MS), and identification of novel disease-specific biomarkers.  相似文献   

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