一种基于fMRI激活实验数据分析的新方法

多种有关用统计学原理来分析fMRI数据这方面的方法已经被提出,并且得到了广泛的应用。这些分析方法的目的是为了产生一幅图像以用于确定任务相关的显著信号变化区。本文提出了一种控制—参考—频率法,该方法通过对时间序列的谱密度进行非参数估计来测试任务频率和血液动力学响应之间的关系,从而达到激活区定位的目的。之后本文通过分析同一组fMRI数据将这种方法和统计参数映射法和相关法进行了比较。实验结果证明了本文所提出的方法在探测由于运动任务所产生的激活区方面是有效的。该方法非常适合探测刺激任务是以周期序列的形式产生时的激活区。

冻干狂犬病疫苗热原检测在HL-60单核细胞激活实验中的方法转移和验证研究

目的研究人早幼粒白血病HL-60单核细胞激活实验在人狂犬疫苗冻干人用狂犬病疫苗热原检测中的可行性。方法将已建立的HL-60单核细胞激活实验进行实验室间方法转移,并进行方法验证;参照《中国药典》细菌内毒素检查法中光度测定法中的干扰试验,用HL-60-IL-6单核细胞激活实验检测13批冻干人用狂犬病疫苗中的回收率及其热原含量。结果以不同浓度内毒素标准品刺激HL-60细胞导致细胞分泌IL-6的量计算与内毒素浓度的线性,R^(2)均为0.95以上;计算最低检测限不超过0.125 EU·mL^(-1);以内毒素含量为0.5、1.0 EU·mL^(-1)的溶液做回收实验,考察方法的准确度;通过HL-60-IL-6检测13批冻干人用狂犬病疫苗,内毒素的回收率均在50%~200%;对4批热原检查、内毒素含量测定不合格的冻干人用狂犬病疫苗和附带的3批注射用水,该方法检测结果与家兔热原检查法和内毒素测定法的结果一致。结论以IL-6为检测指标的HL-60单核细胞激活实验适用于冻干人用狂犬病疫苗的热原物质检测。

应用电教媒体激活化学实验教学探

CAI的灵魂是教学思想,CAI的具体实施是为教学目的服务的。本文尝试运用电教媒体技术优化化学实验教学,创造愉快的学习环境,激发学生学习兴趣,提高教学效率。

酵母表达质粒pGBKT7-hPROKR2-Ct的构建及hPROKR2C端蛋白的自激活鉴定

目的:检测Y2HGold酵母株中表达的h PROKR2 C端蛋白是否有毒性及自激活,为后期利用酵母双杂交技术研究h PROKR2 C端相互作用蛋白奠定基础。方法:构建酵母双杂交载体p GBKT7-h PROKR2-Ct质粒,将其转入酵母感受态中验证其是否表达并计算转化率;通过观察SD/-Trp平板上酵母菌落生长状态进行h PROKR2 C端蛋白的毒性检测;通过观察SD/-Trp、SDO/-Trp/X、SDO/-Trp/X/Aba平板上酵母菌落生长状态进行h PROKR2 C端蛋白自活性检测。结果:构建了酵母双杂交载体p GBKT7-h PROKR2-Ct,将其转入酵母感受态中,转化率为8.5×104cfu/μg;毒性及自活性检测均显示h PROKR2 C端蛋白对酵母菌株无毒性、不具有自活性。结论:可以利用酵母双杂交系统研究hPROKR2 C端相互作用蛋白。

磁分离技术和纳米金比色法用于嗜碱性粒细胞活化试验研究

嗜碱性粒细胞活化试验是一种安全、高效的诊断过敏疾病技术,成为临床体外诊断过敏疾病的主要方法之一。目前,嗜碱性粒细胞活化试验主要是利用流式细胞术对细胞进行检测,这种方法通常存在检测时间长、操作繁琐和成本高等缺点。针对这些问题,本研究开发了一种表面修饰HLA-DR抗体的磁珠分离体系,将其与过敏患者的外周血共孵育5 min后,利用磁性分离技术,筛选出表面含有HLA-DR标记物的细胞。测试结果表明,筛选后的嗜碱性粒细胞在全血中的细胞占比从0.2%提升到11.5%,嗜碱性粒细胞活化试验检测灵敏性得到了有效提高。进一步地,本研究构建了CD63适配体修饰的金纳米粒子检测体系,利用CD63适配体特异性识别活化后的嗜碱性粒细胞表面的CD63抗体,使金纳米粒子在嗜碱性粒细胞表面聚集,溶液颜色由红色转变为蓝紫色,实现对激活的嗜碱性粒细胞可视化比色检测,为临床开展嗜碱性粒细胞活化试验提供了新的方法。

Tetrandrine inhibits activation of rat hepatic stellate cells in vitro via transforming growth factor-β signaling

AIM: To investigate the effect of various concentrations of tetrandrine on activation of quiescent rat hepatic stellate cells (HSCs) and transforming growth factor-β (TGF-β) signaling in vitro.METHODS: HSCs were isolated from rats by in situperfusion of liver and 18% Nycodenz gradient centrifugation, and primarily cultured on uncoated plastic plates for 24 hwith DMEM containing 20% fetal bovine serum (FBS/DMEM) before the culture medium was substituted with 2% FBS/DMEM for another 24 h. Then, the HSCs were cultured in 2% FBS/DMEM with tetrandrine (0.25, 0.5, 1,2 mg/L, respectively). Cell morphological features were observed under an inverted microscope, smooth muscleα-actin (α-SMA) was detected by immunocytochemistry and image analysis system, laminin (LN) and type Ⅲprocollagen (PCⅢ) in supernatants were determined byradioimmunoassay. TGF-β1 mRNA, Smad 7 mRNA and Smad 7 protein were analyzed with RT-PCR and Western blotting, respectively.RESULTS: Tetrandrine at the concentrations of 0.25-2 mg/L prevented morphological transformation of HSC from the quiescent state to the activated one, while α-SMA, LN and PCⅢ expressions were inhibited. As estimated by gray values, the expression of α-SMA in tetrandrine groups (0.25, 0.5, 1, 2 mg/L) was reduced from 21.3% to 42.2%(control: 0.67, tetrandrine groups: 0.82, 0.85, 0.96, or 0.96, respectively, which were statistically different from the control, P＜0.01), and the difference was more significant in tetrandrine at 1 and 2 mg/L. The content of LN in supernatants was significantly decreased in tetrandrine groups to 58.5%, 69.1%, 65.8% or 60.0% that of the control respectively, and that of PCⅢ to 84.6%, 81.5%,75.7% or 80.7% respectively (P＜0.05 vs control), with no significant difference among tetrandrine groups. RTPCR showed that TGF-β1 mRNA expression was reduced by tetrandrine treatments from 56.56% to 87.90% in comparison with the control, while Smad 7 mRNA was increased 1.4-4.8 times. The TGF-β1 mRNA and Smad 7 mRNA expression was in a significant negative correlation (r= -0.755, P＜0.01), and both were significantly correlated with α-SMA protein expression (r = -0.938, P＜0.01;r = 0.938, P＜0.01, respectively). The up-regulation of Smad 7 protein by tetrandrine (1 mg/L)was confirmed by Western blotting as well.CONCLUSION: Tetrandrine has a direct inhibiting effect on the activation of rat HSCs in culture. It up-regulates the expression of Smad 7 which in turn blocks TGF-β1 expression and signaling.

Activation of Landslides in the South of Ukraine under the Action of Natural Seismic Impacts （Experimental and Analytical Studies）

Activation of seismic activity in the Vrancha area, in the Black Sea region resulted in considerable activation of landslides and in increasing of landslide hazard in earthquake-prone areas of Ukraine. Totally about 23,000 landslides were identified in the territory of Ukraine. Experimental and analytical studies of slumps in the Central Livadia landslide system were carried out with the aid of the ZSUV monitoring system. Experimental data were obtained concerning impact of natural seismic factors on the Central Livadia landslide system and on the Palace itself. The South-East wing of the Livadia Palace continuously vibrates relative to a certain midposition. The increase of the amplitude of the faqade deviation from the midposition may be caused by activation of slopes as a result of additional subsidence and ground water rise due to local earthquakes in the Black Sea and because of some other factors.

体外人源细胞激活试验法应用于4种染发剂的皮肤变态反应研究

目的研究体外人源细胞激活试验h-CLAT法应用在染发剂的皮肤变态反应检测中的可行性,通过和现行化妆品标准中体内皮肤变态反应法的比较,评价体外人源细胞激活试验应用在染发剂皮肤变态反应试验上的优劣。方法参考OECD指导原则442E的体外人源细胞系激活试验方法,应用流式细胞仪技术在类树突样的人源白血病细胞系THP-1上对4种染发剂进行体外皮肤变态反应检查,并与体内皮肤变态反应法的检测结果相比较。结果体外h-CLAT试验表明,4种染发剂中#2,#3和#4染发剂的CD54RFI都<200且CD86RFI<150,即体外试验结果为阴性与体内皮肤变态反应试验比较,结果一致;而#1染发剂为体外结果阳性,且有效致敏浓度为315μg·m L-1,与体内变态反应阴性结果不同。结论与体内皮肤变态反应试验相比,体外人源细胞系激活试验在对染发剂的检验上有周期短、测试方法简便、评价结果客观等优点。缺点是无法反映整个过敏反应的过程,存在假阳性的可能。

5种中药有效部位的抗肿瘤作用

目的:研究5种中药有效部位的抗肿瘤作用及机制。方法:通过细胞病变效应法(CPE)、CCK-8法(CCK-8)和肿瘤病毒抗原激活实验系统,观察5种中药有效部位对肿瘤细胞的细胞毒作用和对肿瘤病毒早期抗原表达的抑制作用。结果:5种中药有效部位在一定的剂量范围内,对Hela细胞、EC-109细胞、MCF-7细胞、Bel-7402这4种不同的肿瘤细胞株均有直接的抑制作用,但抑制率有所差异;同时对肿瘤病毒早期抗原基因的表达也均有明显的抑制作用,抑制率在71.2%-94.4%之间。结论:阻断促癌因素也是防治肿瘤的重要手段和方法。结果提示这些中药有效部位可能是通过细胞毒作用和抑制肿瘤病毒抗原表达和基因复制来达到抗肿瘤的作用。

基于THP1-Blue^(TM) NF-κB报告基因法的体外热原检测方法开发与验证

目的:利用导入核因子κB(nuclear factor kappa-B,NF-κB)报告基因和分泌型胚胎碱性磷酸酶(secreted alkaline phosphatase,SEAP)活性的人单核细胞白血病细胞系THP-1细胞,建立一种可用于体外热原检测的方法,并考察方法的可行性和品种适用性。方法:参照《中华人民共和国药典》四部通则9101分析方法验证和9301注射剂安全检查法应用指导原则(附单核细胞活化反应测定法),以细菌内毒素国家标准品作为基准,对THP1-BlueTM NF-κB报告基因法进行专属性、精密度、耐用性等方法学研究;以精密度和阈值作为方法可行性分析的判断指标;并进行品种适用性研究。结果:所建立的方法符合《中华人民共和国药典》9301中单核细胞活化反应测定法的要求,R2均为0.999以上;计算最低检测限0.03 EU·mL^(-1);以内毒素含量为0.5,1.0 EU·mL^(-1)的溶液做回收实验,方法的准确度分别为101%和106%;通过本方法完成人凝血酶原复合物、冻干人纤维蛋白原、b型流感、23价肺炎、牛痘疫苗的品种适用性研究。结论:THP1-Blue^(TM) NF-κB报告基因法满足单核细胞激活实验要求,可用于体外热原物质检测。