人源志贺菌毒力大质粒体外转移及致病性分析

目的为了解志贺菌毒力大质粒能否在体外转移及其转移后是否仍具有致病性。方法将人源福氏志贺菌及其毒力大质粒分别与鸡源鲍氏志贺菌混合,并在37℃培养箱和4℃冰箱中混合培养24 h;用不同剂量的毒力大质粒转移菌株通过口服和腹腔注射分别人工感染雏鸡和小白鼠。结果人源福氏志贺菌的毒力大质成功转移到丢失自身毒力大质粒的鸡源鲍氏志贺菌中;转移菌株对雏鸡和小白鼠均有致病性,且转移菌株的培养特性也有所改变。结论当志贺菌的毒力大质粒裸露出来且具有适宜的条件时,可以在体外转移到相近的病原菌中,且新生成的转移菌株具有一定稳定性和致病性;志贺菌的高致病性需要有毒力大质粒和菌体的其他特殊致病因子同时存在才能完成。

复方苦参注射液对人肝癌SMMC-7221细胞体外增殖、转移和侵袭的抑制作用及其机制

目的探讨复方苦参注射液(CKI)对体外培养的人肝癌SMMC-7221细胞增殖、转移和侵袭的抑制作用及机制。方法用不同稀释百分比〔0.0%(细胞对照组),2.5%,5.0%和10.0%〕的CKI与SMMC-7221细胞共孵育24 h,分别采用MTT法检测细胞存活,采用划痕修复实验和Transwell实验观察细胞迁移和侵袭能力。用5.0%和10.0%的CKI处理SMMC-7221细胞12或24 h后,RT-PCR及Western印迹法分别检测细胞NF-κB mRNA和蛋白的表达水平。结果经2.5%,5.0%和10.0%CKI处理24 h后,SMMC-7221细胞存活率分别为细胞对照组的(92±8)%,(77±5)%(P<0.01)和(56±7)%(P<0.01);细胞迁移率分别为(90±7)%,(50±10)%(P<0.01)和(25±5)%(P<0.01);体外细胞侵袭率分别为(98±7)%,(51±10)%(P<0.01)和(20±5)%(P<0.01)。另外,5.0%和10.0%CKI处理细胞12 h后,NF-κB mRNA水平分别降低至细胞对照组的(42±9)%和(46±10)%(P<0.01),而5.0%和10.0%CKI处理24 h后,NF-κB蛋白表达水平分别降低至(67±16)%和(27±11)%(P<0.01)。结论 CKI具有抑制SMMC-7221细胞增殖、体外转移和侵袭的能力,其机制可能与抑制NF-κB信号通路有关。

微波消融联合经皮骨成形术在椎外溶骨性转移瘤中的应用

目的观察CT引导下微波消融(MWA)联合经皮骨成形术(POP)治疗椎体外溶骨性转移瘤的疗效与安全性。方法回顾性分析接受MWA联合POP治疗18例椎体外溶骨性转移瘤患者的临床资料。采用疼痛视觉模拟量表(visual analogue scale,VAS)、国际肌肉骨骼肿瘤学会(musculo-skeletal tumor society system,MSTS)评分、骨转移患者生活质量特异性量表(QLQ-BM22)评估患者手术前后疼痛程度、肢体功能状态和生活质量;记录手术成功率和术中、术后并发症情况,并对随访期间患者局部肿瘤控制状况和生存期进行统计分析。结果18例患者的MWA联合POP手术均成功。术中4例患者出现少量骨水泥渗漏,均无明显症状。手术前后VAS评分总体差异有统计学意义(F=41.74,P<0.01);术后各时间点VAS评分均低于术前(均P<0.01),而术后各时间点间差异均无统计学意义(均P>0.05)。手术前后MSTS评分总体差异有统计学意义(F=12.40,P<0.01);术后各时间点MSTS评分均高于术前(均P<0.01),而术后各时间点间差异均无统计学意义(均P>0.05)。手术前后QLQ-BM22评分总体差异有统计学意义(F=16.26,P<0.01);术后各时间点QLQ-BM22评分均低于术前(均P<0.01),而术后各时间点间差异均无统计学意义(均P>0.05)。术后随访3~28个月,生存时间为(9.14±7.94)个月。随访期间死亡7例,6例术后1年内死亡,1例术后26个月死亡。3例患者分别于术后8、15、16个月肿瘤复发,平均复发时间为13个月。结论CT引导下MWA联合经皮骨成形术治疗椎体外溶骨性转移瘤并发症少,安全可行,能有效缓解疼痛,改善患者肢体功能,提高患者运动能力和生活质量,术后局部肿瘤复发率低且复发周期较长。

经皮骨成形术治疗92例肺癌椎体外骨转移患者的临床观察

目的 :探讨经皮骨成形术治疗肺癌椎体外骨转移患者的安全性和临床疗效。方法 :2008年6月—2012年12月,92例肺癌椎体外骨转移患者接受经皮骨成形术。于术前24 h以及术后24 h、1个月、3个月和6个月时,采用视觉模拟评分评定患者疼痛缓解情况,采用Karnofsky体能状况评分和活动能力评分评定患者生活质量改善情况。对于骨盆转移患者,采用Harris髋关节评分评定髋关节功能恢复情况;对于四肢转移患者,采用Mirels评分评定四肢骨折风险改善情况。结果 :92例患者均顺利完成手术,手术成功率为100%,未发生严重并发症。术后患者的疼痛、生活质量、活动能力和髋关节活动功能均有明显改善,四肢骨折风险有所下降,其中术前24 h与术后1个月和3个月时的各类相关评分的差异均有统计学意义(P<0.05)。结论 :经皮骨成形术治疗肺癌骨转移患者的手术创伤较小,可以明显缓解患者的疼痛,提高患者的生存质量,值得在临床上推广应用,但应注意选择合适的患者及手术时机。

肿瘤微环境双重响应性水飞蓟宾纳米胶束体外抗乳腺癌活性及转移研究

肿瘤微环境的复杂特征为肿瘤治疗带来考验的同时也为新型治疗策略提供了新的途径。本研究合成了肿瘤微环境pH响应和谷胱甘肽(glutathione,GSH)响应的聚(2-乙基-2噁唑啉)-聚乳酸-二硫键聚β氨基酯[poly(2-ethyl-2-oxazoline)-poly(lactic acid)-SS-poly(β-amino ester),PEOz-PLA-SS-PBAE]三嵌段共聚物,通过薄膜水化法负载水飞蓟宾(silybin)制备胶束,以提高水飞蓟宾抗肿瘤活性。通过芘荧光探针法测定该聚合物的临界胶束浓度(critical micelle concentration,CMC)为1.8μg·mL^(-1)。动态光散射法测定胶束粒径为155.30±1.80 nm,多分散指数(polydispersity index,PDI)为0.168±0.004。HPLC测定胶束的载药量和包封率为(5.48±0.04)%和(68.52±0.48)%。其体外释放结果表现出胶束具有pH与GSH敏感性,具有缓释效果。通过测定空白胶束的溶血率和细胞毒性试验证明材料具有良好的生物相容性。载药胶束组细胞毒性实验和细胞凋亡实验表明PEOz-PLA-SS-PBAE载药胶束对MDA-MB-231细胞具有显著的抑制效果和诱导其凋亡的效果。细胞划痕实验与Transwell侵袭实验结果显示PEOz-PLA-SS-PBAE载药胶束能够显著抑制MDA-MB-231细胞的转移。因此,本研究制备的PEOz-PLA-SS-PBAE载药胶束具有良好的体外抑制肿瘤生长以及抗肿瘤转移的作用,为水飞蓟宾的进一步应用铺垫了基础。

蛋白磷酸酶Ⅰ(PPP1R3)在直肠癌细胞体外侵袭转移的生物学活性研究

目的探讨研究蛋白磷酸酶I(protein phosphatase1 regulatory subunit 3,PPP1R3)在直肠癌SW480细胞中的黏附、运动、迁移和侵袭能力的生物学活性。方法用PPP1R3、EGFR抗体、VEGFR抗体干预SW480细胞后,分别对其行细胞运动实验、黏附实验、迁移及侵袭实验,分析PPP1R3对SW480细胞运动、黏附、迁移和侵袭能力的影响及其作用机制。结果随着PPP1R3浓度的增加,直肠癌SW480细胞的黏附、运动、迁移和侵袭能力明显减退(P<0.05)。而且穿过人工基底膜的能力明显减低(P<0.05)。结论 PPP1R3能够抑制直肠癌SW480体外的侵袭、转移作用,可为PPP1R3基因表达缺失的直肠癌术后患者提供放化疗、生物靶向治疗依据。

2型重组腺相关病毒/增强型绿色荧光蛋白转染胰腺癌细胞PANC-1的体外研究

基因治疗的关键是目的基因的高效转染和表达。我们采用2型重组腺相关病毒（rAAV2／EGFP）对人胰腺癌细胞PANC-1进行体外基因转移，观察EGFP基因能否在PANC-1中有效表达及其细胞毒性，探讨rAAV2介导目的基因转导胰腺癌细胞的效率。

Preliminary Observation on the Influence of Tumor Osseous Metastasis on Autologous Peripheral Blood Stem Cell Collection

OBJECTIVE To examine the influence of tumor osseous metastasis on the patients undergoing autoiogous peripheral blood stem ceil collection. METHODS A total of 36 patients with malignant diseases who received an autoiogous peripheral blood stem ceil transplantation, during a period from April 2004 to June 2006, were chosen. The patients were divided into two groups, i.e. group A were patients with a complication of tumor osseous metastasis, and group B were without metastasis. Both groups were treated with Taxotere 120 mg/m^2 plus granuiocyte colony-stimulating factor （G-CSF） 5 μg/kg/d, for a mobilization regimen. A blood ceil separator was used to collect the mononuciear ceils. The proportion of harvested CD34＋ ceils in the peripheral blood and the collected mononuciear ceils were detected by flow cytometry. The number of CD34＋ ceils was used to determine the difference in the nature of the collections between the two groups. RESULTS After mobilization in groups A and B, the number of the peripheral blood mononuciear ceils （PBMC） was 39.3±14.7% and 41.1±12.4 % and the proportion of CD34＋ ceils was 0.16±0.07% and 0.17±0.10%, respectively. Following administration of the drugs, there was no significant difference between the number of harvested PBMC and CD34＋ cells of the two groups, i.e., 3.47±1.16×10^8/Kg and 2.52±1.43×10^6/Kg in group A and 4.02±1.31×10^8/Kg and 2.73±1.87×10^6/Kg in group B, respectively. CONCLUSION Osseous metastasis, as a single factor, may have no impact on mobilization and harvesting of hematopoietic stem ceils and their engraftment after autotransplantation.

Role of VEGF-A/C and CCR-7 in the enhanced metastasis of A549 cells induced by 2 and 4 Gy X-rays in vitro and in vivo

Radiotherapy is a common strategy in treating lung cancer.Accumulating evidence suggested that radiotherapy has the potential to promote the metastasis and invasion of carcinoma cells.In this study,we aimed to testify the role of vascular endothelial growth factor(VEGF)and C-C chemokine receptor-7(CCR-7)in the metastasis of human adenocarcinoma A549 cells in vivo and in vitro.Nude mice were injected with A549 cells irradiated by 0,2 and 4 Gy X-rays,respectively.Quantitative detections of VEGF-A/C and CCR-7 mRNA from lung sample were performed by real-time RT-PCR.Small interfering RNA(siRNA)transfection technology was further used to testify the role of the genes in the metastasis of A549 cells.VEGF and CCR-7mRNA could only be detected 10 weeks post injection in vivo when visible tumor foci scattered in lung.In addition,VEGF-A/C mRNA expressed significantly higher in mice injected with A549 cells irradiated by 2 and 4 X-rays than those with 0 Gy X-rays irradiation.On the other hand,A549 cells with or without X-rays irradiation transfected with VEGF siRAN and CCR-7 siRNA showed a dramatic decrease of invasiveness compared to normal A549 cells with or without irradiation.The migration indexes were?0.7,?0.48,?0.34 and?0.32 for A549 cells with CCR-7 siRNA,VEGF siRNA,X-rays combined CCR-7 siRNA and X-rays combined VEGF-siRNA respectively.These results demonstrated that X-rays could promote the metastasis of A549 cells,and VEGF-A/C and CCR-7 mRNA were closely related to the metastasis of A549 cells in vivo and in vitro.