lncRNA TP53TG1在牙髓中的表达和对牙髓干细胞转录炎症因子的影响

目的探究lncRNA TP53TG1在健康和炎症牙髓中的表达差异,以及对脂多糖(LPS)诱导后人牙髓干细胞(hDPSCs)炎症因子转录水平的影响。方法设计合成lncRNA探针,利用RNA荧光原位杂交技术检测健康和炎症牙髓组织中lncRNA TP53TG1的表达情况。通过酶解组织块法分离培养hDPSCs,对培养的hDPSCs进行多向分化诱导验证,并通过流式细胞术鉴定表型特征。将hDPSCs分为si-NC组、si-NC+LPS组、si-TP53TG1+LPS组,分别转染对照序列和TP53TG1的siRNA,再用LPS处理si-NC+LPS组和si-TP53TG1+LPS组24 h,通过qRT-PCR检测各组炎症因子IL-1β、IL-8以及TNF-α的mRNA表达水平。结果在健康牙髓组织中可观察到lncRNA TP53TG1的表达,主要分布在成牙本质细胞中。炎症状态下,lncRNA TP53TG1的表达量上升,全牙髓可见分布。LPS处理后,hDPSC的TNF-α、IL-1β以及IL-8的mRNA表达水平上升,下调lncRNA TP53TG1导致hDPSCs的TNF-αmRNA表达水平进一步升高。结论lncRNA TP53TG1可能参与调控牙髓炎症过程和成牙本质细胞的免疫调控作用。

lncRNA TP53TG1在结肠癌中的表达及通过mi R-18a/CDC42轴对癌细胞发展的影响

目的:探讨lncRNA TP53TG1通过miR-18a/CDC42轴对SW620细胞发展的影响。方法:分析结肠癌组织、癌旁组织、SW620、NCM460细胞中lncRNA TP53TG1、miR-18a和CDC42的表达。检测下调TP53TG1对细胞增殖、侵袭和上皮间质转化(EMT)的影响。采用生物信息学miRanda分析LncRNA TP53TG1作用靶点,检测TP53TG1和miR-18a的相关性。检测下调miR-18a或上调LncRNATP53TG1通过miR-18a对细胞增殖、侵袭和EMT的影响。TargetScan分析miR-18a靶点,检测miR-18a和CDC42之间的关系。分析CDC42 siRNA对细胞增殖、侵袭和EMT的影响。结果:和癌旁正常组织相比,结肠癌组织中lncRNA TP53TG1和CDC42表达上调,miR-18a表达下调;和NCM460细胞相比,SW620细胞中lncRNA TP53TG1和CDC42表达上调,miR-18a表达下调。lncRNA TP53 TG1 siRNA或CDC42 siRNA抑制细胞增殖、侵袭与EMT;lncRNA TP53TG1靶向miR-18a,miR-18a靶向CDC42。miR-18a inhibitor促进细胞增殖、侵袭与EMT;上调LncRNATP53TG1通过miR-18a促进CDC42表达和细胞发展。结论:lncRNA TP53TG1在结肠癌中表达上调且通过miR-18a/CDC42轴促进SW620细胞增殖、侵袭及其EMT。

A candidate protective factor in amyotrophic lateral sclerosis:heterogenous nuclear ribonucleoprotein G

Heterogenous nuclear ribonucleoprotein G is down-regulated in the spinal cord of the Tg(SOD1*G93A)1Gur(TG)amyotrophic lateral sclerosis mouse model.However,most studies have only examined heterogenous nuclear ribonucleoprotein G expression in the amyotrophic lateral sclerosis model and heterogenous nuclear ribonucleoprotein G effects in amyotrophic lateral sclerosis pathogenesis such as in apoptosis are unknown.In this study,we studied the potential mechanism of heterogenous nuclear ribonucleoprotein G in neuronal death in the spinal cord of TG and wild-type mice and examined the mechanism by which heterogenous nuclear ribonucleoprotein G induces apoptosis.Heterogenous nuclear ribonucleoprotein G in spinal cord was analyzed using immunohistochemistry and western blotting,and cell proliferation and proteins(TAR DNA binding protein 43,superoxide dismutase 1,and Bax)were detected by the Cell Counting Kit-8 and western blot analysis in heterogenous nuclear ribonucleoprotein G siRNA-transfected PC12 cells.We analyzed heterogenous nuclear ribonucleoprotein G distribution in spinal cord in the amyotrophic lateral sclerosis model at various time points and the expressions of apoptosis and proliferation-related proteins.Heterogenous nuclear ribonucleoprotein G was mainly localized in neurons.Amyotrophic lateral sclerosis mice were examined at three stages:preonset(60-70 days),onset(90-100 days)and progression(120-130 days).The number of heterogenous nuclear ribonucleoprotein G-positive cells was significantly higher in the anterior horn of the lumbar spinal cord segment of TG mice at the preonset stage than that of control group but lower than that of the control group at the onset stage.The number of heterogenous nuclear ribonucleoprotein G-positive cells in both central canal and surrounding gray matter of the whole spinal cord of TG mice at the onset stage was significantly lower than that in the control group,whereas that of the lumbar spinal cord segment of TG mice was significantly higher than that in the control group at preonset stage and significantly lower than that in the control group at the progression stage.The numbers of heterogenous nuclear ribonucleoprotein G-positive cells in the posterior horn of cervical and thoracic segments of TG mice at preonset and progression stages were significantly lower than those in the control group.The expression of heterogenous nuclear ribonucleoprotein G in the cervical spinal cord segment of TG mice was significantly higher than that in the control group at the preonset stage but significantly lower at the progression stage.The expression of heterogenous nuclear ribonucleoprotein G in the thoracic spinal cord segment of TG mice was significantly increased at the preonset stage,significantly decreased at the onset stage,and significantly increased at the progression stage compared with the control group.heterogenous nuclear ribonucleoprotein G expression in the lumbar spinal cord segment of TG mice was significantly lower than that of the control group at the progression stage.After heterogenous nuclear ribonucleoprotein G gene silencing,PC12 cell survival was lower than that of control cells.Both TAR DNA binding protein 43 and Bax expressions were significantly increased in heterogenous nuclear ribonucleoprotein G-silenced cells compared with control cells.Our study suggests that abnormal distribution and expression of heterogenous nuclear ribonucleoprotein G might play a protective effect in amyotrophic lateral sclerosis development via preventing neuronal death by reducing abnormal TAR DNA binding protein 43 generation in the spinal cord.

高密度培养大肠杆菌TG1/pGEX-hCT和高表达重组人降钙素

目的 :高密度、高表达培养重组大肠杆菌 TG1/p GEX- h CT,生产重组人降钙素 (rh CT)。 方法和结果 :应用 NBSBio Flo30 0 0型 5 L 自控发酵罐 ,采用分批培养和补料分批培养相结合的培养技术 ,控制碳源和氮源的补加 ,控制溶解氧 ,使重组菌 E.coli TG1/p GEX- h CT发酵光密度 [D(6 0 0 ) ]达到 5 8.6 ,人降钙素和 GST融合蛋白 (GST- h CT)的含量达到 3.2 g/L。结论 :本研究为工业化生产重组 h CT奠定了基础。

电穿孔法转化大肠杆菌TG1的条件优化

研究了质粒pFab74X经电穿孔转化大肠杆菌TG1菌株的影响因素 ,并优化其转化条件。电场强度和脉冲时间的影响较为复杂 ,两者适当组合才可获得高转化效率。此外 ,采用对数生长早期的细菌 。

健胃愈疡颗粒对消化性溃疡患者胃黏膜IL8和TGFβ1表达的影响

目的:观察健胃愈疡颗粒(柴胡、党参、白芍、延胡索、白及、甘草等)对消化性溃疡患者胃黏膜IL8和TGFβ1表达的影响,探讨健胃愈疡颗粒的疗效机制。方法:56例胃溃疡(肝郁脾虚证)患者,随机分为治疗组和西药对照组,另设正常对照组;治疗组予健胃愈疡颗粒;对照组予法莫替丁片加硫糖铝片,4周为1个疗程,HP阳性者加用阿莫西林胶囊和甲硝唑片;治疗前后胃镜下取溃疡边缘黏膜活检。免疫组化及RT-PCR检测TGFβ、IL8表达水平;结果:(1)IL8在正常胃黏膜中呈阴性或偶有阳性表达,治疗前两组表达高于正常组(P<0.01),治疗后均减少至接近正常水平,两组无显著性差异(P>0.05)。(2)TGFβ1在正常胃黏膜中有少量表达,两组治疗前较正常胃黏膜增加,两组间差异无显著性(P>0.05);治疗后两组表达均显著增加,且治疗组高于对照组(P<0.05);结论:健胃愈疡颗粒可能通过抑制炎性细胞因子IL8的表达,增强促溃疡愈合因子TGFβ1的表达,达到促进溃疡愈合的目的。

大肠埃希菌TG_1电穿孔法转化条件优化研究

为了确立稳定的高效率电转化方案,提高构建文库的库容,分别对细菌培养温度、生长状态、电场强度、感受态细胞浓度和体积、外源基因的质量、甘油/甘露醇缓冲液体积等条件进行优化,分析了各因素对转化效率的影响。结果显示:细菌培养温度为16℃,细菌生长的OD_(600)值为0.5,密度梯度离心洗涤法,感受态细胞浓度高于1×10^(11)/m L,并设定电场强度14.25 k V/cm时进行电穿孔,转化效率最高,可达到9×10~9CFU/μg DNA。研究获得的电转化优化条件为高库容文库的构建提供了一个重要的途径。

长链非编码RNA-TP53TG1在神经胶质瘤细胞中对糖剥夺应激反应的影响

目的构建长链非编码RNA-TP53TG1的真核表达克隆,并探索其在神经胶质瘤中对糖剥夺应激反应的影响。方法用RT-PCR方法从人胶质瘤细胞中扩增出TP53TG1;构建了TP53TG1的全长真核表达克隆;实时定量PCR检测其在U87MG细胞内的表达;同时用低糖(0.3 g/L葡萄糖、8 h)处理;real-time PCR检测GRP78、IDH1和PKM2的表达水平。结果成功构建了真核重组表达质粒pCIG-TP53TG1;在转染U87MG细胞36 h后,可见绿色荧光的表达,U87MG细胞中TP53TG1 mRNA升高了2.9×106倍(P<0.05);过表达TP53TG1的同时低糖处理,GRP78和IDH1 mRNA的表达水平显著升高(P<0.05),而PKM2 mRNA的表达水平显著降低(P<0.05)。结论在U87MG细胞中,TP53TG1可能通过影响GRP78、IDH1和PKM2 mRNA的表达,而参与到对糖剥夺的应激反应过程。

调控TGFβ1/SMAD通路的microRNAs在失神经支配骨骼肌中的表达

目的：本研究拟探讨骨骼肌失神经支配后差异性表达的microRNAs,并明确其是否参与调控TGFβ1/SMAD信号通路.方法：C57/BL6J小鼠,随机分为正常对照组和实验组,实验组小鼠切断右下肢坐骨神经为手术组,左下肢游离坐骨神经作为假手术组.4周后处死小鼠取腓肠肌Masson染色观察肌纤维形态变化,比较各组肌纤维横截面积.以TGFβ1/SMAD为靶基因,通过生物信息学分析寻找到18个可能的miRNAs指标.定量PCR检测其表达,并针对表达升高的microRNAs采用荧光素酶报告基因实验确认其靶基因.结果：手术组肌纤维横截面积比对照组明显缩小,对照组与假手术组肌肉之间的差异无统计学意义.在失神经骨骼肌中特异性高表达的有miR-424、miR-744、miR-15a.在C2C12细胞系中行报告基因实验显示,与对照组比较,转染miR-744后,SMAD3的荧光素酶强度下降;转染miR-15a后,TGFβ1的荧光素酶强度下降;转染miR-424后,SMAD3的荧光素酶强度变化无统计学意义.PCR验证microRNAs的靶基因显示,转染miR-744、miR-15a的模拟物后,分别对应的SMAD3、TGFβ1表达下调,差异有统计学意义.结论：miR-424、miR-744、miR-15a可能参与调控失神经支配导致的骨骼肌萎缩纤维化,其中miR-744的靶基因是SMAD3,miR-15a的靶基因是TGFβ1.

Tg1／P91钢的发展应用及其焊接性综述

本文对Tg1／P91钢的发展概况、发展现状、焊接过程后产生裂纹与冲击韧性下降的问题进行了综述和分析。就如何焊接缺陷和裂纹等问题进行了初步的讨论，并且对国内T91／Pg1生产的现状和存在的问题进行了总结，为如何获得优质的焊接接头进行了总结，希望为我国电力大直径厚壁管的焊接提供参考。

电转化条件对大肠杆菌TG1转化效率的影响

研究探索不同条件对TG1大肠杆菌转化率的影响,以探索最适合电转化条件。研究通过对细菌生长曲线绘制,改变不同生长阶段、感受态细胞浓度、转化后复苏液以及复苏时间、电转化参数、质粒浓度、抗生素浓度等影响电转化率的条件,探索最适合的电转化条件。结果表明,TG1大肠杆菌37℃、170 rpm/min震荡活化培养时间3 h后,以电压1 800 V、电容25μF、电阻200Ω进行电击转化,以LB液体对电击细胞复苏45 min,为最佳转化条件。该结果具有可重复性,为后续建立基因文库奠定良好基础。

Genesis of Low-Resistivity Oil layers from Cretaceous System in Luxi Area and Its Geological Significance

Genesis of low resistivity oil layers from cretaceous system in Luxi area was studied. The result shows that the resistivity of oil layers is lower than that of water layers from Tugulu Group(K 1tg),Cretaceous in Luliang area,Zhungeer basin, resulting in a disaccordance with logging interpretation on oil layers,oil water layers and water layers?The research on the petro texture of reservoirs also shows that the watered clay pellicle (I/S, I, ch) is well developed in K 1tg expands the section of conductive net and results in a low resistivity of oil layers.

ITU-R/TG8/1第16次会议简介

一、会议概况ＩＴＵ－Ｒ／ＴＧ８／１第１６次会议于１９９９年３月８日到３月１９日在巴西ＦＯＲＴＡＬＡＺＡ召开，会议注册登记的代表共有２００多位，来自３３个国家，４个国际组织和若干生产厂商。我国派出了由１１人组成较大规模的代表团。信息产业部科技司的闻库副...

Phosphoinositide-3-kinase regulatory subunit 4 participates in the occurrence and development of amyotrophic lateral sclerosis by regulating autophagy

The development of amyotrophic lateral sclerosis(ALS)may be related to the abnormal alterations of multiple proteins.Our previous study revealed that the expression of phosphoinositide-3-kinase regulatory subunit 4(PIK3R4)was decreased in ALS.However,the role of PIK3R4 in ALS pathogenesis remains unknown.This study was the first to find that transfection of PC12 cells with small interfering RNA against the PIK3R4 gene significantly decreased the expression levels of PIK3R4 and the autophagy-related proteins p62 and LC3.Additionally,in vivo experiments revealed that the PIK3R4 protein was extensively expressed in the anterior horn,posterior horn,central canal,and areas surrounding the central canal in cervical,thoracic,and lumbar segments of the spinal cord in adult mice.PIK3R4 protein was mainly expressed in the neurons within the spinal lumbar segments.PIK3R4 and p62 expression levels were significantly decreased at both the pre-onset and onset stages of ALS disease in Tg(SOD1*G93A)1 Gur mice compared with control mice,but these proteins were markedly increased at the progression stage.LC3 protein expression did not change during progression of ALS.These findings suggest that PIK3R4 likely participates in the prevention of ALS progression.This study was approved by the Ethics Committee for Animal Care and Use of Jiangxi Provincial People’s Hospital,Affiliated People’s Hospital of Nanchang University(approval No.2020025)on March 26,2020.

德国耐驰推出全新热重分析仪

德国耐驰仪器公司推出全新的热重分析仪TG209F1。它与差示扫描量热仪DSC204F1一起，由于其全新的独特设计，构成了理想的新一代热分析仪器系列。热重分析(TG)为使样品处于程序控制的温度下，测量样品的质量随温度与时间的变化过程。它是一种进行质量控制与失效分析的理想工具。

EFFECTS OF HERBAL CAKE-SEPARATED MOXIBUSTION ON BLOOD LIPIDS, PLASMA THROMOXANE B2 AND 6-KETO-PROSTAGLANDIN F_(1α) CONTENTS IN THE RABBIT WITH HYPERLIPEMIA

Objective: To observe effects of herbal cake-separated moxibustion on blood lipids, including total cholesterol (TCh), triglyceride (TG), high density lipoprotein-Ch (HDL-Ch), low density lipoprotein-Ch (LDL-Ch), apolipoprotein A (Apo A), apolipoprotein B (Apo B), and plasma thromboxane B2 (TXB2) and 6-keto-prostaglandin F 1α (6-keto-PGF 1α) contents and analyse its mechanism. Methods: The hyperlipemia rabbit model was established by breeding of high fat forage and injection of bovine serum albumin. They were treated respectively by direct moxibustion and herbal cake-separated moxibustion at Juque (巨阙 CV 14), Tianshu (天枢 ST 25), Fenglong (丰隆 ST 40), etc., once daily, continuously for 40 days. Blood TCh and TG contents were detected with enzymatic method, LDL-Ch and HDL-Ch with colorimetric method, Apo A and Apo B with electrophoretic method, and TXB2 and 6-keto-PGF 1α with radioimmunoassay. Results: Both the herbal cake-separated moxibustion and direct moxibustion could effectively decrease TCh, TG, LDL-Ch, Apo B and TXB2 contents and TXB2/6-keto-PGF 1α, and increase HDL-CH and 6-keto-PGF 1α contents in the rabbit of hyperlipemia. Conclusion: 6-keto-PGF 1α and TXB2 are possibly involved in the mechanism of herbal cake-separated moxibustion decreasing blood lipids.