修复抑制剂对不同辐射敏感性作物生物学效应的影响

本文研究了辐射损伤修复抑制剂咖啡因、ＥＤＴＡ后处理对不同辐射敏感性作物大豆和油菜生物学效应的影响。结果表明，辐射与咖啡因、ＥＤＴＡ后处理对两种作物幼苗的发芽率没有明显的影响；除低剂量（大豆＜１００Ｇｙ，油菜＜６００Ｇｙ）辐照具有刺激生长作用外，两种作物幼苗的根长、苗高、干物重和ＩＡＡ含量均随辐照剂量的增大而逐渐降低；咖啡因、ＥＤＴＡ后处理进一步降低了幼苗的根长、苗高和干物重，但缓解了ＩＡＡ含量的下降水平。咖啡因、ＥＤＴＡ及其复合后处理对两种作物根长、苗高和干物重的影响程度表现为：咖啡因＋ＥＤＴＡ＞咖啡因＞ＥＤＴＡ。

修复抑制剂对侧耳辐射损伤的效应

侧耳双核菌丝经γ射线辐照后用咖啡因或Ｎａ＿２－ＥＤＴＡ处理，其生长速度和漆酶及多酚氧化酶活性较单一γ射线辐照明显降低，使辐射损伤加剧；辐照前用咖啡因和Ｎａ＿２－ＥＤＴＡ处理，抑制辐射损伤修复的效果优于辐照后处理；咖啡因和Ｎａ＿２－ＥＤＴＡ浓度分别达到０．５和１．０ｍｇ／ｍＬ后，单独处理侧耳菌丝会直接引起生理损伤。用咖啡因和Ｎａ＿２－ＥＤＴＡ抑制侧耳辐射损伤修复，从而提高诱变效率是可行的。最适浓度以不直接引起生理损伤的最高浓度为宜，咖啡因和Ｎａ＿２－ＥＤＴＡ适宜浓度分别为０．２和０．５ｍｇ／ｍｌ．咖啡因的效果优于Ｎａ＿２－ＥＤＴＡ。

甲氧胺联合手霉素对白血病U937细胞凋亡的影响

背景与目的:DNA损伤修复对细胞生存很重要。我们既往的研究发现手霉素可诱导肿瘤细胞出现DNA损害反应。因此,碱基切除修复抑制剂甲氧胺(methoxyamine)有可能增强手霉素(manumycin)的抗肿瘤作用。为此,本实验研究甲氧胺对手霉素诱导白血病细胞凋亡的影响,探讨联合甲氧胺和手霉素诱导白血病细胞凋亡过程中线粒体凋亡途径的变化。方法:不同浓度手霉素和甲氧胺处理U937细胞48h后,MTT细胞毒性测定U937细胞存活率,软琼脂法检测细胞的克隆形成。应用流式细胞术检测细胞凋亡。免疫印迹技术检测细胞色素C、Caspase-9、聚腺苷核糖聚合酶(poly-adenosyl ribose polymerase,PARP)的表达。中位效应方法评价两药的相互作用。结果:甲氧胺使手霉素的剂量反应曲线向左边移动,结合指数(CI)<1(P<0.05)。1μmol/L手霉素、5mmol/L甲氧胺和联合两药处理U937细胞,相对于对照组的克隆形成分别是0.3641±0.0463,0.7541±0.0379,0.0473±0.0024(联合用药组与对照组、手霉素组或甲氧胺组相比,P<0.05);进一步发现,联合两药协同诱导细胞凋亡,引起Annexin V荧光值增加,阳性细胞增加,分别是(2.34±0.30)%、(8.80±0.95)%、(2.21±0.19)%、(13.37±0.91)%,联合用药组与对照组、手霉素组或甲氧胺组相比,差异有统计学意义(P<0.05)。联合甲氧胺和手霉素增强细胞色素C从线粒体释放到细胞浆,Caspase-9激活,PARP特异性裂解。结论:甲氧胺增强手霉素通过线粒体凋亡途径诱导U937细胞凋亡,提示甲氧胺联合FTIs和DNA修复抑制剂治疗白血病的可能性。

DNA修复与肿瘤的耐药

化疗药物是临床治疗肿瘤的常见方法,但其先天性和获得性耐药也是临床亟需解决的问题。肿瘤细胞DNA修复能力的改变是引起该类药物产生耐药的重要因素之一。DNA修复是维持基因组稳定的主要因素,一种DNA损伤可能被多种DNA修复通路修复。了解DNA修复与化疗药物耐药性之间的关系,开发DNA修复抑制剂联合化疗可以克服化疗药物的耐药性并提高临床效果,同时为临床合理运用化疗药物及研制低耐药性药物提供理论依据。

Veliparib联合青蒿琥酯体外抗细粒棘球蚴作用机制的研究

目的观察DNA损伤修复抑制剂Veliparib联合青蒿琥酯体外对细粒棘球蚴活性的影响,分析Veliparib联合青蒿琥酯抗囊型包虫病的作用机制。方法将细粒棘球蚴分为空白组,DMSO组,Veliparib(10μmol/L)组,硝唑尼特(nitazoxanide,NTZ)组,H2O2组,青蒿琥酯低(65μmol/L)、中(130μmol/L)、高(325μmol/L)剂量组,H2O2+Veliparib组,青蒿琥酯低剂量+Veliparib组,青蒿琥酯中剂量+Veliparib组、青蒿琥酯高剂量+Veliparib组,共12组。采用1%伊红染色法检测药物干预2、3、4d细粒棘球蚴的活性,计算虫体死亡率。给药组干预细粒棘球蚴4d后,观察虫体组织病理学和超微结构变化;通过彗星试验评价DNA损伤情况;采用免疫荧光法观察虫体内DNA损伤标志物8-羟基脱氧鸟苷(8-oxo-dG)的变化。结果与DMSO组和青蒿琥酯各剂量组相比,青蒿琥酯低、中、高剂量联合Veliparib组细粒棘球蚴死亡率均显著升高(P<0.01);组织病理学观察青蒿琥酯各剂量联合Veliparib组细粒棘球蚴虫体损坏情况较青蒿琥酯各剂量组严重且明显固缩,着色加深,并有空泡形成;超微结构观察青蒿琥酯各剂量联合Veliparib组的细粒棘球蚴合胞体带混沌,细胞结构破坏,异染色质边际化,出现脂滴、空泡样结构,微绒毛明显破坏或减少;彗星试验显示青蒿琥酯各剂量联合Veliparib组细粒棘球蚴彗星拖尾较低、中、高青蒿琥酯组明显加长,Olive尾矩(OTM)值差异均有统计学意义(t值分别为5.358,2.482和4.224,P<0.05)。免疫荧光显示青蒿琥酯高剂量+Veliparib组8-oxo-dG的阳性核数较青蒿琥酯高剂量组增多。结论 DNA损伤修复抑制剂Veliparib增强青蒿琥酯抗囊型包虫病作用,其作用机制是使虫体的DNA损伤更严重,从而导致棘球蚴死亡,为开发新的抗包虫病药物奠定了理论基础。

Effect of nitric oxide synthase inhibitor on proteoglycan metabolism in repaired articular cartilage in rabbits

Objective: To study the effect of nitric oxide synthase inhibitor, S-methyl thiocarbamate (SMT), on proteoglycan metabolism in repaired articular cartilage in rabbits. Methods: Twenty-four male New Zealand white rabbits, aged 8 months and weighing 2.5 kg±0.2 kg, were used in this study. Cartilage defects in full thickness were created on the intercondylar articular surface of bilateral femurs of all the rabbits. Then the rabbits were randomly divided into 3 groups (n=8 in each group). The defects in one group were filled with fibrin glue impregnated with recombinant human bone morphogenetic protein-2 (rhBMP-2, BMP group), in one group with fibrin glue impregnated with rhBMP-2 and hypodermic injection with SMT (SMT group) and in the other group with nothing (control group). All the animals were killed at one year postoperatively. The tissue sections were stained with safranine O-fast green and analyzed by Quantiment 500 system to determine the content of glycosaminoglycan through measuring the percentage of safranine O-stained area, the thickness of cartilages and the mean gray scale (average stain intensity). Radiolabelled sodium sulphate ( Na 2 35SO 4) was used to assess the proteoglycan synthesis. Results: At one year postoperatively, the percentage of safranine O-stained area, the mean gray scale and the cartilage thickness of the repaired tissues in SMT group were significantly higher than those of BMP group (P< 0.01) and the control group (P< 0.05). Result of incorporation of Na 2 35SO 4 showed that the proteoglycan synthesis in SMT group was higher than those of BMP group and the control group (P< 0.01). Conclusions: SMT, a nitric oxide synthase inhibitor, can significantly increase the content of glycosaminoglycan and proteoglycan synthesis, and computer-based image analysis is a reliable method for evaluating proteoglycan metabolism.