Effect of long non-coding RNA MEG3 on invasion and migration of colorectal cancer cells

AIM: To investigate the expression of long non-coding RNA maternally expressed gene 3(MEG3) in colorectal cancer(CRC) cells, and to observe the effect of MEG3 on the invasion and migration of CRC cells. METHODS: The levels of MEG3 in human normal colon cell NCM460 and CRC cells SW48 and LoVo were detected by real- time PCR. MEG3 was over-expressed by plasmid transfection, and the effects of MEG3 on the invasion and migration of SW48 and LoVo cells were analyzed by Transwell assay and wound healing assay. The expression of matrix metalloproteinase(MMP) family proteins was determined by Western blotting. RESULTS: The level of MEG3 was down-regulated in CRC cells compared with normal colon cell NCM460. The invasion and migration of CRC cells were reduced after MEG3 over-expression. Transwell invasion and migration assays showed that the numbers of transmembrane SW48 and LoVo cells were smaller in MEG3 over-expression group than control group(CONCLUSION: The expression of MEG3 is down-regulated in CRC cells. Over-expression of MEG3 inhibits the invasion and migration of CRC cells. TIMP-2, MMP-2 and MMP-9 might play an important role in this regulation.     

Antineurotoxic activity of Galactia glaucescens against Crotalus durissus terrificus venom

Ethanolic extract of leaves of Galactia glauscescens (GGE) at concentration of 100 and 500 mug/ml prevented the neuromuscular paralysis induced by Crotalus durissus terrificus venom on mouse phrenic nerve-diaphragm preparation.     

湖南永州尖吻蝮蛇蛇毒的蛋白组分及毒性分析

采用Nano–LC–ESI–MS/MS蛋白鉴定技术对湖南永州尖吻蝮蛇蛇毒蛋白组分进行质谱分析,应用常规体外试管法对尖吻蝮蛇蛇毒体外溶血值进行检测,采用改良寇式法对尖吻蝮蛇蛇毒LD_(50)进行测定。结果显示:尖吻蝮蛇蛇毒含有50种蛋白,蛋白相对分子质量集中在1.0×10~4～2.0×10~4(46.9%)、4.0×10~4～5.0×10~4(22.4%)、2.0×10~4～3.0×10~4(10.6%)和7.0×10~4～8.0×10~4(7.6%),其中代表性的高丰度蛋白有蛇毒金属蛋白酶A(11.7%)、蛇毒金属蛋白酶H1(9.8%)、蕲蛇类凝血酶–2(7.3%)、抗凝血酶A–A亚基(6.8%),低丰度蛋白(0.1%)有Ecto–5'–核苷酸酶、碱性磷脂酶A2 DAV–N6、生长分化因子11;蛇毒引起红细胞溶血的最低质量浓度为60.00μg/mL,尖吻蝮蛇蛇毒对KM小鼠的LD_(50)为7.1796mg/kg,攻毒小鼠出现呼吸急促、躁动不安、注射部位出现奇特瘙痒和大面积溃烂,至死亡。     

白色霞水母刺细胞毒素抗烟草花叶病毒活性

为探索从水母毒素中获取抗植物病毒物质的应用前景,采用半叶枯斑法、整株法和漂浮叶圆片法,对白色霞水母Cyanea nozakii Kishinouye刺细胞毒素的抗烟草花叶病毒(Tobacco mosaic virus,TMV)活性进行了检测。结果表明,白色霞水母刺细胞毒素对TMV具有很强的直接钝化作用,枯斑抑制率随钝化时间的延长而增大。0.99 mg/m L毒素体外钝化TMV 30 min,枯斑抑制率达98.85%,将TMV与0.80 mg/m L毒素体外混合后立即接种,枯斑抑制率仍达89.57%;20~70℃之间,毒素对TMV的钝化作用随温度升高而降低,但又表现出一定的高温耐受性,70℃下处理30min,1.33 mg/m L毒素对枯斑的抑制率为61.73%。毒素对病毒初侵染有一定的预防作用,并可抑制TMV的增殖;1.93 mg/m L毒素处理接种TMV的叶圆片2 d后,对TMV的增殖抑制率为49.41%;但该毒素对TMV所致病害的治疗效果不明显。该毒素还具有较强的蛋白水解酶活性,可能与其抗TMV活性相关。表明白色霞水母刺细胞毒素抗TMV作用明显,其抗植物病毒活性值得深入研究。     

持续被动运动通过抑制软骨细胞NO合成下调MMP-1和MMP-13表达

目的：观察持续被动运动（CPM）和补充一氧化氮（NO）供体——硝酸甘油（NG）对兔骨关节炎（OA）模型中软骨基质金属蛋白酶-1（MMP-1）和MMP-13表达以及NO含量的影响，探讨CPM下调MMPs的可能机制。方法：30只3~4月龄雄性新西兰大白兔，其中6只进行假手术作为正常对照组（NC组），另外24只建立膝关节OA模型，术后随机分为4组，即OA对照组（OA组）、OA硝酸甘油给药组（NG组）、OA持续被动运动组（CPM组）、OA持续被动运动+硝酸甘油给药组（CPM+NG组），每组各6只。NC组和OA组不作处理，NG组给予NG软膏膝关节局部涂抹，CMP组在CPM训练仪上进行膝关节持续被动运动，CMP+NG组即在运动干预的同时给予NG局部涂抹。4周后取各组软骨组织，硝酸还原酶法测定NO含量，HE染色观察软骨形态学变化并进行Mankin''s评分，实时荧光定量PCR（RQ-PCR）检测MMP-1和MMP-13 mRNA水平，免疫组织化学法测定MMP-1和MMP-13蛋白表达量。结果：NO含量、Mankin''s评分以及MMP-1和MMP-13 mRNA和蛋白水平在OA组明显高于NC组（P<0.01），NG组高于OA组（P<0.01），CPM组低于OA组和NG组（P<0.01），CPM+NG组低于NG组（P<0.01），但高于CPM组（P<0.01）。结论：CPM通过抑制软骨细胞NO合成下调MMP-1和MMP-13表达，进而对软骨细胞起保护作用。     

MMP-2、MMP-9在子宫内膜增生症和腺癌中的表达

目的 探讨基质金属蛋白酶-2(MMP-2)和MMP-9在子宫内膜腺癌发生、发展中的作用.方法 采用免疫组化法检测100例子宫内膜腺癌、30例子宫内膜增生症及30例正常子宫内膜中MMP-2、MMP-9表达.结果 MP-2、MMP-9 在正常子宫内膜增生期表达增加,而在早分泌期几乎无表达;MMP-2、MP-9在不典型增生及...     

GVF Snake模型在木材表面缺陷分割的应用研究

针对木材表面存在纹理、凹凸结构、边缘颗粒和弱边缘等特点,对其直接运用Snake模型进行分割难以得到有效边缘提取,因此提出运用改进的GVF Snake模型和维纳滤波相结合对其进行分割。首先对木材图像进行维纳滤波使得纹理变得平缓,同时可以使得缺陷边缘得到有效保留,再对其进行GVF Snake模型分割。该算法对初始轮廓的选择敏感度降低,拓展性增强,可以使得轮廓曲线更加快速地收敛到缺陷边缘,避免陷入局部最优现象,提高对弱边缘和凹凸图像分割效果,分割结果更加清晰、连贯,具有良好的实时性。为木材表面缺陷的分割提供一种更为有效的方法,拓宽了snake模型的应用范围。     

Effects of pirenzepine on expression of MMP-2 and TIMP-2 in stroma of sclera in chick myopic eyes

AIM:To observe the effect of intravitreal injection of pirenzepine on form-deprivation myopia in chicks. METHODS:Forty-one day old chicks were randomly divided into 4 groups:normal control group, form deprivation group, vehicle control group and pirenzepine injection group. The right eyes of all chicks were used as experimental eyes. The deprived eyes in vehicle control group and pirenzepine injection group received daily intravitreal injection of vehicle control solution(0.01 mol/L PBS) and pirenzepine(1%in PBS), respectively. Optical examinations such as refraction, axial length and equatorial diameter were made at the end of the 5th day. The mRNA and protein levels of matrix metalloproteinase 2(MMP-2) and tissue inhibitor of metalloproteinase-2(TIMP-2), and the activity of MMP-2 were detected by RT-PCR, Western blotting and zymography analysis,respectively. RESULTS:Refraction, axial length and equatorial diameter of the eyes in pirenzepine injection group were significantly lower than those in form deprivation group and vehicle control group(P<0.05), but those were higher(P<0.05) and the eyes were relatively myopic as compared with normal control group. The mRNA expression, protein le vels and activity of MMP-2 in pirenzepine group were significantly higher than those in normal control group(P<0.01), and were significantly lower than those in form deprivation group and vehicle control group(P<0.01, P<0.01). The mRNA and protein levels of TIMP-2 in pirenzepine group were significantly lower than those in normal control group(P<0.01), and was significantly higher than those in form deprivation group and vehicle control group(P<0.01, P<0.01). CONCLUSION:Intravitreal injection of pirenzepine may partly prevent form-deprivation myopia by modulating the expression of MMP-2 and TIMP-2 in the fibrous layer of sclera.