线粒体脑肌病伴乳酸血症和卒中样发作综合征的临床特征及遗传学研究

目的探讨线粒体脑肌病伴乳酸血症和卒中样发作（MELAS）综合征临床与分子遗传学特征,寻找MELAS线粒体DNA（mtDNA）A3243G点突变比例与临床特征的关联性。方法对2001年1月至2008年1月在首都医科大学附属北京儿童医院神经内科住院和门诊临床疑似线粒体脑肌病的患儿,行外周血白细胞mtDNA A3243G点突变筛查、血乳酸检测和神经影像学等检查。A3243G点突变阳性病例中选取符合MELAS临床疑似诊断标准的患儿（突变阳性组）,对其家系进行调查,采集家族成员血进行mtDNA A3243G点突变筛查;A3243G点突变阴性病例中选取符合MELAS临床疑似诊断标准的患儿行肌肉病理活检和肌肉A3243G点突变筛查（突变阴性组）。分析比较两组的临床资料及MELAS遗传学特征。结果研究期间共有272例疑似线粒体脑肌病的患儿进行了外周血白细胞A3243G点突变的筛查。A3243G点突变的20例阳性标本中,突变均为异胞质性（heteroplasmy）,18例符合MELAS的临床疑似诊断标准。血细胞中突变型mtDNA的比例为9.0%-50.0%,其中4例同时在肌肉组织检测到相同突变,突变比例为42.4%-64.8%。临床症状以惊厥、乏力、智力进行性倒退、发热、呕吐、视力障碍和失语为主,身材矮小和体毛增多为主要体征,13例合并癫,血乳酸均升高,头颅CT/MRI显示双侧对称性苍白球钙化和脑梗死信号。A3243G点突变筛查阴性标本中有4例临床符合MELAS临床疑似诊断标准,肌肉病理可见破碎红边纤维,肌肉A3243G点突变筛查阴性。14个家庭中的37名家庭成员采集了外周血进行mtDNA A3243G点突变筛查,突变阳性组中患儿母亲5名检测到A3243G点突变,突变比例分别为3.0%,5.0%,11.8%,21.3%和26.9%,同胞兄弟4名检测到A3243G突变,突变比例分别为19.3%、33.3%,37.5%和41.5%,均无临床症状,其他成员未检测到突变。本研究A3243G点突变比例与发病年龄和就诊年龄呈负相关趋势,与病程未?     

Binding of Cellular Proteins to the Leader RNA of Equine Arteritis Virus

The genome of equine arteritis virus (EAV) produces a 3 coterminal-nested set of six subgenomic (sg) viral RNAs during virus replication cycle, and each set possesses a common leader sequence of 206 nucleotides (nt) in length derived from the 5 end of the viral genome. Given the presence of the leader region within both genomic and sg mRNAs, it is likely to contain cis-acting signals that may interact with cellular or viral proteins for RNA synthesis. Gel mobility shift assays indicated that proteins in Vero cell cytoplasmic extracts formed complexes with the positive (+) and negative (-) strands of the EAV leader RNA. Several cell proteins with molecular masses ranging from 74 to 31 kDa and 58 to 32 kDa were detected in UV-induced cross-linking assays with the EAV leader RNA (+) and (-) strands, respectively. In both cases, intense bands were observed at the 58–52 kDa molecular weight markers. Results from competition gel mobility shift assays using overlapping cold RNA probes spanning the leader RNA (+) strand indicated that nt 140–206 are not necessary for binding to cell proteins.     

Engulfment of mast cell secretory granules on skin inflammation boosts dendritic cell migration and priming efficiency

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壳聚糖醋酸溶液对凝血作用的研究

研究了不同脱乙酰度和不同分子量壳聚糖醋酸溶液的凝血作用。发现壳聚糖醋酸溶液使抗凝血液中红细胞发生了明显的聚集和变形。通过不同分子量和脱乙酰度壳聚糖的促红细胞聚集实验,证明了低脱乙酰度壳聚糖(60%~70%)使红细胞聚集效果更好,分子量在105~106范围内作用不十分明显。对血液的凝血酶时间(TT)、凝血酶原时间(PT)、活化部分促凝血酶原激酶时间(APTT)和纤维蛋白原浓度(FIB)的测定结果验证了壳聚糖醋酸溶液凝血机理不依赖于血小板和常规“瀑布”凝血机制。     

Juvenile sudden death in a family with polymorphic ventricular arrhythmias caused by a novel RyR2 gene mutation: evidence of specific morphological substrates

We report on a family with a history of sudden death and effort-induced polymorphic ventricular arrhythmias. The index case was a 17-year-old boy who died suddenly and at postmortem had evidence of fibrofatty replacement in the right ventricular free wall, consistent with arrhythmogenic right ventricular cardiomyopathy, as well as calcium phosphate deposits within the myocytes. A molecular genetics investigation carried out in the paraffin-embedded myocardium of the subject and in blood samples of family members disclosed a missense mutation in exon 3 (230C-->T; A77V) of the cardiac ryanodine receptor type 2 gene. The carriers showed effort-induced polymorphic ventricular tachycardia in the setting of normal resting electrocardiogram and trivial echocardiographic abnormalities, consistent with catecholaminergic polymorphic ventricular tachycardia. The observation of both arrhythmogenic right ventricular cardiomyopathy type 2 and catecholaminergic polymorphic ventricular tachycardia in the same family suggests that the two entities might correspond to different degrees of phenotypic expression of the same disease. This experience underscores the importance of a precise autopsy diagnosis in the case of sudden cardiac death, including molecular genetics, and the mission of pathologists to guide further clinical investigation of family members.     

酪氨酸酶基因在HEK293细胞表达的MRI评价

目的:以酪氨酸酶基因作为报告基因转染HEK293细胞, 利用其合成大量黑色素而能被MRI检测的特性来反映基因表达的情况, 以探索磁共振成像(MRI)评价体外细胞基因表达的方法。方法:以脂质体将含酪氨酸酶基因完全cDNA的pcDNA3tyr质粒转染到HEK293细胞, 以MRIT₁WI、T₁WI/SPIR、T₂WI序列扫描转染细胞, 观察表达的黑色素的MRI信号。应用Fontana染色检测黑色素的合成, RT-PCR检测酪氨酸酶基因的cDNA片段, 以进一步验证酪氨酸酶基因的转染与表达。结果:(1)pcDNA3tyr质粒转染进入HEK293细胞并在其中表达生成黑色素, 转染5μg、10μg、20μg质粒的10⁶个细胞内生成的黑色素能够被MRI检测到并在MRIT₁WI、T₁WI/SPIR、T₂WI检查呈高信号, MRI信号强度与转染质粒量成正相关。(2)Fontana染色法检测到HEK293细胞内的黑色素颗粒;(3)采用RT-PCR方法检测到转染的HEK293细胞含酪氨酸酶基因的cDNA片段。结论:MRI能够检测到HEK293细胞内由外源基因表达合成的黑色素, 说明影像学与分子生物学技术结合可以评价体外细胞基因表达的情况。     

Setting out the frame conditions for feasible use of FFPE derived RNA

Introduction

The usage of formalin-fixed paraffin embedded (FFPE) tissue is characterized by its long shelf-life and simple handling. Therefore it is the most commonly available tissue specimen in routine diagnostics and histological studies. Formaldehyde fixation may result in RNA degradation and cross linking with proteins, while storage conditions also affect RNA integrity. The present study was designed to investigate the influence of these factors on RNA analysis.

Plastid genomes of the Rhodophyta and Chromophyta constitute a distinct lineage which differs from that of the Chlorophyta and have a composite phylogenetic origin,perhaps like that of the Euglenophyta

Summary A phylogenetic tree has been constructed from comparisons of entire 16S rRNA gene sequences from different prokaryotes and from several algal plastids. According to this study, and to previous work on the ribulose-1,5-bisphosphate carboxylase oxygenase (Rubisco) large and small subunit genes, we postulate that: (1) rhodophyte and chromophyte plastid genomes have a common, composite phylogenetic origin which implies at least two different ancestors, a cyanobacterial and a -proteobacterial ancestor; (2) chlorophyte (green algae and land plants) plastids have a cyanobacterial ancestor which probably differs from that of rhodophyte and chromophyte plastids, and in any case constitute a different lineage; (3) euglenophyte plastid genomes also seem to have a composite phylogenetic origin which involves two different lineages.     

鞭毛抗原与细菌的群集运动

群集运动是指在培养基表面某些运动细菌依赖鞭毛的群体迁移行为,涉及繁殖体细胞分化成群集细胞,发生形态、代谢以及蛋白表达等显著变化。菌细胞密度、表面接触和生理学信号均可成为群集运动的刺激因素。群集运动的关键是鞭毛的生物合成,flhDC鞭毛操纵子是支配分化和迁移的细菌调控网络的焦点。     

Detection of numerical chromosomal abnormalities in malignant cells on body fluids by fluorescence in situ hybridization of interphase cell nuclei with chromosome-specific probes.

To detect numerical chromosomal abnormalities (NCA) in malignant cells on body fluids, Fluorescence in situ hybridization (FISH) technique was tested in clinical specimens from patients with metastatic disease. Directly labeled DNA probes specific for chromosomes 8, 12, X, and Y (Imagenetics, Naperville, IL) were used for in situ hybridization to interphase cell nuclei. Fifteen body fluids (BF) from various sites were studied. Based initially on the Papanicolaou-stained slides, there were seven malignant and eight benign samples. Blind analysis (200 cells/sample) showed that all benign samples had a normal number of chromosomes, whereas six of seven malignant samples showed different NCA comprising 5-60% of the cell population ranging from three to 10 chromosome signals per cell. We conclude that interphase cytogenetic cell analysis of BF by FISH is: (1) feasible and gives superior signals for detection of NCA, (2) helpful in detecting malignant cells, (3) relatively simple with a turnaround time of less than 24 hr. This method may have diagnostic and prognostic application in the study of the biologic behavior of malignant neoplasms.