HER-2阳性乳腺癌靶向治疗进展

乳腺癌是女性最常见的癌症,同时也是第二大致死性的癌症。人表皮生长因子受体2(human epidermal growth factor receptor-2,HER-2)阳性乳腺癌是具有侵袭性的乳腺癌亚型,预后差,复发率高。HER-2是一个可用于治疗的靶标,针对HER-2基因的研究,开发不同的靶向治疗药物,在临床上取得了很好的治疗效果。本文结合文献介绍了目前已经获批的靶向药的作用机制和疗效,以及正在研究的新型靶向药,包括新型酪氨酸激酶抑制剂(ONT-380),新抗体-药物偶联物(MM-302)的进展。

miR-3941抑制securin的表达对神经胶质瘤细胞的影响

目的探讨miR-3941对神经胶质瘤发生发展的影响以及可能的分子机制。方法为了明确miR-3941的功能,本研究将细胞分为三组,一组不做任何处理(U251细胞组),一组转染NC mimics作为对照组(NC mimics组),一组转染miR-3941 mimics(miR-3941 mimics组)。为了研究securin对miR-3941功能的影响,又将细胞分为三组,一组转染miR-3941 mimics(miR-3941 mimics组),一组共转染miR-3941 mimics和空质粒作为对照(miR-3941mimics+NC组),一组共转染miR-3941 mimics和securin过表达质粒(miR-3941 mimics+ov-securin组)。采用RTqPCR检测人正常胶质细胞和胶质瘤U251细胞中miR-3941的表达情况。CCK-8实验和Transwell实验检测过表达miR-3941、过表达miR-3941同时过表达securin对胶质瘤U251细胞增殖、迁移和侵袭影响。Western blot检测过表达miR-3941、过表达miR-3941同时过表达securin对胶质瘤U251细胞中securin蛋白表达的影响。双荧光素酶报告实验分析miR-3941对securin的靶向作用关系。结果与人正常胶质细胞相比,胶质瘤U251细胞中miR-3941相对表达水平显著下调,差异有统计学意义(t=57.42,P<0.05)。CCK-8实验表明在培养48和72 h时U251细胞组、NC mimics组以及miR-3941 mimics组之间细胞增殖差异有统计学意义(F=424.50、956.20,P均<0.05);miR-3941 mimics组的增殖明显低于NC mimics组(P<0.05)。Transwell实验表明U251细胞组、NC mimics组以及miR-3941 mimics组的细胞迁移和侵袭差异有统计学意义(F=6361.00、5608.00,P均<0.05);和NC mimics组相比,转染miR-3941mimics组迁移和侵袭细胞数显著减少(P<0.05)。双荧光素酶实验结果显示,与野生型securin 3’-UTR报告载体共转染后,U251组、miR-3941 mimics组和miR-3941 inhibitor组之间荧光素酶活性差异有统计学意义(F=649.10,P<0.05),而与突变后的securin 3’-UTR报告载体共转染后,以上三组荧光强度无明显变化,差异无统计学意义(F=0.55,P=0.605)。Western blot检测发现转染miR-3941 mimics的胶质瘤U251细胞中securin蛋白水平明显降低。miR-3941 mimics组、miR-3941 mimics+NC组以及miR-3941 mimics+ov-securin组在48和72 h时间点细胞增殖差异有统计学意义(F=541.40、516.80,P均<0.05),三组细胞迁移和侵袭差异有统计学意义(F=3611.00、9684.00,P均<0.05)。与miR-3941 mimics+NC组相比,miR-3941 mimics+ov-securin组细胞的增殖、迁移和侵袭能力均显著增强(P均<0.05)。结论miR-3941可通过抑制securin的表达抑制神经胶质瘤的发生发展。

In vivo perfusion staining of atherosclerotic lesions and a novel quantification method for lesion size in sequential aortic root sectioning in murine models

Objectives To develop a simple, accurate and reproducible method, which combines macro and histopathological techniques for determining the degree of lipid deposition in genetically modified mice. Method The entire aortas from C57BL/6, ldlr-/- and apoE-/- mice were stained with Sudan IV using either in vivo perfusion or traditional in vitro enface staining techniques. Histological sections of aortic root and hearts were embedded in tissue freezing medium and cut with a cryostat, then stained with Oil Red O. The calculated aortic root area based on the aortic root circumference was used to reduce measurement errors. Results The in vitro en face staining can stain all fat, which include the adventitial tissue around aorta. However the in vivo perfusion staining can specifically stain the fatty deposition inside of aorta. Both entire aorta and aortic root section staining showed that there was a highly significant increase in fatty deposition in the aortas of the genetic modified mice. Although all mice genetic background was same, the apoE-/- mice had larger atherosclerotic lesions than ldlr-/- mice. Conclusions The new in vivo peffusion method is more accurate than the in vitro en face method. The combination of these macro and microscopic techniques overcomes the shortcomings of the earlier published methods which are generally limited to the measurement of fatty red staining areas only, neglecting non-specific adventitial fat staining around aorta and aortic root section tissue distortion.