TGIF 对胃癌细胞生长和转移的影响

TGIF (TG-interacting factor) 是 TGF- β信号传导通路的抑制分子, 而 TGF-β早期抑制肿瘤生长,晚期促进肿瘤浸润与转移,但 TGIF 在肿瘤发生中的作用尚不清楚 . 将 TGIF 基因稳定转染胃癌细胞株 SGC-7901 ,采用 MTT 法、平板克隆形成试验、流式细胞术和裸鼠成瘤试验探讨 TGIF 对胃癌细胞生物学行为的影响,通过免疫组织化学分析裸鼠瘤组织基质金属蛋白酶 (matrix metallo proteinases, MMP) MMP2 、 MMP9 和血管内皮生长因子 (vascular eudothelial growth factor, VEGF) 的表达,通过 ELISA 和明胶酶谱试验分别分析 TGIF 转染细胞上清液中 VEGF 和活性 MMP2 与 MMP9 的含量变化 . TGIF 对 SGC-7901 细胞的生长、细胞周期分布和克隆形成率无影响 . TGIF 转染细胞接种裸鼠后无癌栓形成,但对照组有癌栓形成,且其瘤组织 MMP9 和 VEGF 的表达明显低于对照组,但 MMP2 在 3 组间的表达无差别 . TGIF 基因转染细胞、 PcDNA3.1 转染细胞和 SGC-7901 细胞上清液中 VEGF 的浓度分别为 (635 ± 20.3) ng/L 、 (780±25.4) ng/L 和 (791±23.9) ng/L , TGIF 转染细胞 VEGF 的含量明显低于对照组细胞 (P <0.01) , TGIF 转染细胞上清液中活性 MMP9 的含量明显低于对照组 . 尽管 TGIF 能部分拮抗 TGF-β1 介导的生长抑制和细胞周期阻滞作用,但它并不能使胃癌细胞的生物学行为恶化,相反 TGIF 通过下调 VEGF 和 MMP9 的表达降低胃癌细胞的浸润与转移能力 .     

抗人尿道高分化鳞癌单克隆抗体的研制

用本室建立的人尿道高分化鳞状上皮癌细胞株(Hus-98)免疫Balb/C小鼠,通过细胞杂交技术及ELISA方法进行筛选,SP免疫组织化学方法进行鉴定,获得10株能稳定分泌、选择性强、效价高的杂交瘤细胞株;同时从乳腺癌组织中提出肿瘤相关抗原行免疫印记实验(Western-blot)。结果6株经4次克隆能稳定分泌抗体Ig,免疫组化显示这些抗体是针对来源于上皮的鳞癌、腺癌细胞膜和细胞浆的,而癌旁正常组织及胎儿组织呈阴性反应;通过western-blot结果显示肿瘤相关抗原分子量为46.414kb。     

Comparison of cytotoxic activities betweenin vitro and field grown plants ofTyphonium flagelliforme (Lodd.) blume

Anin vitro cytotoxicity screening of theTyphonium flagelliforme extracts indicated high cytotoxicity effect on human lung carcinoma NCl-H23 cells and human mammary gland carcinoma T-47D cells, but the extracts were not active on human liver carcinoma HepG2 cells. NCl-H23 cells were more susceptible toT. flagelliforme extracts than T-47D cells. EDP₅₀ values of the hexane fractions of the mature plant and thein vitro plantlet ofT. flagelliforme on NCl-H23 cells were less than 2 μg/mL Extract from the mature plant was relatively more cytotoxic than the one fromin vitro plantlet except for the hexane fraction. The chloroform and butanol fraction of the mature plant had higher cytotoxicity effect than the fraction fromin vitro plantlet on NCl-H23 cells. All the 3 fractions (hexane, chloroform, and butanol) of the mature plant exhibited higher cytotoxicity effects on human mammary gland carcinoma T-47D cells than the 3 fractions ofin vitro plantlet. However, the human liver carcinoma cells were resistant toT. flagelliforme extracts except for higher concentration of hexane fractions of both the mature and thein vitro plants and the chloroform fraction of the mature plant. Micropropagated plantlets ofT. flagelliforme could hence be used as herbal materials for the treatment of human lung and breast cancers.     

Accuracy of touch imprint cytology in diagnosing lung cancer.

A 3-year study assessed the diagnostic accuracy of touch imprint smears in the diagnosis of lung cancer. Touch imprint smears were prepared from 90 computerized tomographic-guided core needle lung biopsies. Cytological diagnosis of touch imprint smears were correlated with the histological diagnosis of the corresponding core needle biopsy specimen, which was taken as the gold standard. The sensitivity, specificity, positive predictive value and negative predictive value of imprint smear results were 89%, 100%, 100% and 68%, respectively. There were no false positives, and all patients with small cell lung cancer were correctly diagnosed with this technique. Imprint cytology can be used to provide a rapid, preliminary diagnosis of lung cancer.     

实验性腹膜炎肺损伤时大黄的保护作用

目的探讨大黄对实验性腹膜炎时肺损伤的保护作用.方法用酵母多糖A腹腔注射制备大鼠急性腹膜炎模型,诱发肺脏损伤.将SD大鼠随机分为4组:(1)正常组,(2)模型组,(3)大黄实验组,(4)抗生素实验组(氨苄西林组).测定肺组织匀浆中丙二醛(MDA)、黄嘌呤氧化酶(XOD)、谷光甘肽(GSH)和血清内毒素水平,并进行血气分析及外周血WBC计数.结果大黄组内毒素、肺组织匀浆中MDA和XOD,以及白细胞计数均明显低于模型组(P＜0.05),而还原GSH变化不明显.结论大黄可能通过降低外周及门静脉血内毒素水平,抑制脂质过氧化和加强自由基的清除,从而减轻实验性腹膜炎引起的肺损伤.     

实验性腹膜炎时内毒素血症及肺脏的变化

目的探讨实验性腹膜炎时,内毒素与肺损伤的变化.方法用酵母多糖A腹腔注射制备大鼠急性实验性腹膜炎模型,随机分为模型组和对照组;观察实验性腹膜炎时,肺损伤变化.结果模型组内毒素、肺匀浆脂质过氧化物,以及白细胞计数均明显增高;而还原谷胱甘肽(GSH)明显降低,与对照组比差异有显著性(P＜0.05).结论实验性腹膜炎时,内毒素的形成、细菌因子的释放及脂质过化与肺损害有一定的联系.     

Physical interaction between Tbx6 and mespb is indispensable for the activation of bowline expression during Xenopus somitogenesis

Crk is a member of a family of adaptor proteins that are involved in intracellular signal pathways altering cell adhesion, proliferation, and migration. Increased expression of Crk has been described in lung cancer and associated with increased tumor invasiveness. MicroRNAs (miRNAs) are a family of small non-coding RNAs (approximately 21–25 nt long) that are capable of targeting genes for either degradation of mRNA or inhibition of translation. Crk is a predicted putative target gene for miR-126. Over-expression of miR126 in a lung cancer cell line resulted in a decrease in Crk protein without any alteration in the associated mRNA. These lung cancer cells exhibit a decrease in adhesion, migration, and invasion. Decreased cancer cell invasion was also evident following targeted knockdown of Crk. MiR-126 alters lung cancer cell phenotype by inhibiting adhesion, migration, and invasion and the effects on invasion may be partially mediated through Crk regulation.     

TLR4 signaling in cancer cells promotes chemoattraction of immature dendritic cells via autocrine CCL20

Toll-like receptors (TLRs) are involved in the production of inflammatory mediators upon specific ligands stimuli. Chemokines are important inflammatory mediators capable of chemoattracting diverse immune cells. In addition to normal immune cells, the expression of TLRs and chemokines has been detected in various tumor cells. However, the roles of TLRs and chemokines expressed by tumor cells in the processes of tumor progression and immune escape have not been fully elucidated. Here we report that TLR4 ligation by lipopolysaccharide (LPS) significantly promotes CT-26 colon cancer cells to produce chemokine CCL20 via activation of TLR4 signaling pathways. We find that LPS treatment of CT-26 cells can significantly increase the chemoattraction of immature dendritic cells (DC) by the autocrine CCL20. Our studies suggest that TLR4 expressed by tumor cells may be involved in the induction of chemokines like CCL20, providing a potential linkage between chronic inflammation and tumor immune escape.