慢病毒介导的外源基因体外投递系统的建立

目的针对不同哺乳类细胞建立相应的慢病毒体外感染体系，以建立慢病毒介导的外源基因体外投递系统。方法按Invitrogen公司推荐的标准程序进行慢病毒（携带EGFP基因）包装（脂质体介导的瞬时转染）、超速离心浓缩和保存等，随后用病毒上清或浓缩后的病毒感染293FT细胞，24—48h后荧光显微镜下观察是否见绿色荧光以证实慢病毒是否成功生产；将携带EGFP基因的病毒上清或浓缩后的病毒分别加入内含293FF细胞、小鼠ES细胞、小鼠胚胎成纤维细胞（MEFs）或小鼠睾丸生殖细胞的培养板孔内，感染6—12h后，用相应培养基替换感染液，数天后荧光显微镜下观察是否见绿色荧光以证实慢病毒是否成功感染不同哺乳类细胞。结果按标准程序生产的携带EGFP基因慢病毒（病毒上清或浓缩后的病毒）成功高效率感染293FF细胞、MEFs或小鼠睾丸生殖细胞；用浓缩后的病毒（携带EGFP基因）感染小鼠ES细胞，亦可获得EGFP阳性的ES细胞克隆。结论熟练掌握了慢病毒包装、浓缩及鉴定等技术，同时针对不同哺乳类细胞建立了相应的慢病毒介导的外源基因体外传递系统，这些为相关后续研究打下了良好的基础。     

PMX2B,a new candidate gene for Hirschsprung's disease

Hirschsprung's (HSCR) disease is a congenital intestinal malformation of the enteric nervous system. It is a multigenic malformation and until now, eight genes have been involved in the etiology of this disease: genes encoding proteins of the RET signaling pathway (RET, GDNF and NTN), genes participating in the endothelin (EDN) type B receptor pathway (EDNRB, EDN3 and ECE-1), the SOX10 gene and the SIP1 gene that is mutated in syndromic forms of HSCR. Mutations of these genes are found in not more than 50-60% of affected individuals. Here, we report on the results of a molecular cytogenetic study performed in a girl who presented with a syndromic short segment HSCR associated with a de novo t(4;8)(p13;p22) translocation. A comparative genomic hybridization (CGH) study found a 4p12p13 deletion. A molecular characterization of this rearrangement showed that the 4p13 deletion was 5 Mb in length and included the paired mesoderm homeobox gene (PMX2B) (MIM 603851), a gene expressed in the human embryonic gut and essential for the development of autonomic neural crest derivatives. The present observation suggests that PMX2B haploinsuffciency might predispose to HSCR.     

Brain prostaglandin formation is increased by α-synuclein gene-ablation during global ischemia

We have previously demonstrated that α-synuclein (Snca) gene ablation reduces brain arachidonic acid (20:4n − 6) turnover rate in phospholipids through modulation of endoplasmic reticulum-localized acyl-CoA synthetase activity. Although 20:4n − 6 is a precursor for prostaglandin (PG), Snca effect on PG levels is unknown. In the present study, we examined the effect of Snca ablation on brain PG level at basal conditions and following 30 s of global ischemia. Brain PG were extracted with methanol, purified on C₁₈ cartridges, and analyzed by LC–MS/MS. We demonstrate, for the first time, that Snca gene ablation did not affect brain PG mass under normal physiological conditions. However, total PG mass and masses of individual PG were elevated ∼2-fold upon global ischemia in the absence of Snca. These data are consistent with our previously observed reduction in 20:4n − 6 recycling through endoplasmic reticulum-localized acyl-CoA synthetase in the absence of Snca, which may result in the increased 20:4n − 6 availability for PG production in the absence of Snca during global ischemia and suggest a role for Snca in brain inflammatory response.     

Duplication of distal 22q

We report on three patients with duplication of distal 22q. One patient is a de novo carrier of the translocation t(21;22) (p13;q11), the other two are offspring of a translocation carrier t(10;22) (q26;q12). The clinical manifestations of these patients demonstrate the variability of the dup(22q) syndrome.     

FISH characterization of a supernumerary r(1)(::cen→q22::q22→sq21::) chromosome associated with multiple anomalies and bilateral cataracts

We describe the case of a 15‐year‐old girl with multiple congenital anomalies, dysmorphic features, severe kyphoscoliosis, growth and mental retardation, and the absence of speech, in whom 35% of the cells carried a supernumerary ring chromosome 1. Fluorescence in situ hybridization (FISH) analysis using YAC/BAC clones spanning the region from 1p13 to 1q21 made it possible to determine the genomic content and structure of the ring(1), which was found to consist of the cytogenetic bands 1q21–22. A complex structure was delineated in the ring chromosome with a partial inverted duplication delimited by markers WI‐7732 and WI‐607, with WI‐7396 and WI‐8386 being the boundaries of the single copy segment. Comparison of the clinical signs of other patients with mosaic r(1) reported in the literature allowed the identification of a patient sharing a number of clinical signs including cataracts. Given that mutations of the GJA8 gene encoding connexin 50 (Cx50) and mapping to 1q21 have been associated with the presence of cataracts, it is possible that a gain in copy number or a rearrangement of GJA8 may contribute to cataractogenesis.     

Molecular analysis in Japanese patients with Charcot-Marie-Tooth disease: DGGE analysis for PMP22, MPZ,and Cx32/GJB1 mutations

Charcot-Marie-Tooth disease (CMT) is a heterogeneous disorder and is traditionally classified into two major types, CMT type 1 (CMT1) and CMT type 2 (CMT2). Most CMT1 patients are associated with the duplication of 17p11.2-p12 (CMT1A duplication) and small numbers of patients have mutations of the peripheral myelin protein 22 (PMP22), myelin protein zero (MPZ), connexin 32 (Cx32/GJB1), and early growth response 2 (EGR2) genes. Some mutations of MPZ and Cx32 were also associated with the clinical CMT2 phenotype. We constructed denaturing gradient gel electrophoresis (DGGE) analysis as a screening method for PMP22, MPZ, and Cx32 mutations and studied 161 CMT patients without CMT1A duplication. We detected 27 mutations of three genes including 15 novel mutations; six of PMP22, three of MPZ, and six of Cx32. We finally identified 21 causative mutations in 22 unrelated patients and five polymorphic mutations. Eighteen of 22 patients carrying PMP22, MPZ, or Cx32 mutations presented with CMT1 and four of them with MPZ or Cx32 mutations presented with the CMT2 phenotype. DGGE analysis was sensitive for screening for those gene mutations, but causative gene mutation was not identified in many of the Japanese patients with CMT, especially with CMT1. Other candidate genes should be studied to elucidate the genetic basis of Japanese CMT patients.     

Inverted tandem (“mirror”) duplications in human chromosomes: Inv dup 8p, 4q, 22q

We have studied 4 patients with inverted tandem duplications of parts of chromosomes, a hitherto rarely identified from of a structural rearrangement involving a single chromosome in man. In Patients 1 and 2, the duplication involved parts of the short arm of chromosome 8 (regions 8p 12→8p23 and 8p21→8p23, respectively). Both patients manifested certain characteristics of the mosaic trisomy 8 syndrome. Elevated levels of glutathione reductase (GSR) in their erythrocytes supported the interpretation of a partial duplication of chromosome 8 and indicated a regional localization for the GSR gene locus. In Patient 3, the distal half of the long arm of chromosome 4 was duplicated (region4q26→4q35). Clinical evidence supported this interpretation, as Patient 3 resembled phenotypically the 13 reported cases with duplication of the distal 4q. The cytogenetic findings in Patient 4 suggested a possibly inverted duplication of 22q. The clinical correlation was less convincing due to the lack of a well-defined phenotype for trisomy 22. These chromosome aberrations had occurred de novo in all 4 cases. Although they involved different chromosomal regions, they might well have arisen by the same mechanism. Possible modes of origin that are discussed in detail include unequal exchange between homologous chromosomes, between chromatids of 1 chromosome or between strands of 1 DNA duplex.     

超高效液相色谱-串联质谱法同时快速检测微量血清中6种脂溶性维生素

目的 建立超高效液相色谱-串联质谱法（UPLC-MS/MS）同时快速检测微量血清中维生素A、维生素D（25-OH-VD2 、25-OH-VD3 ）、维生素E（α-、β-和γ-生育酚）的方法。方法 血清中脂溶性维生素经甲醇-乙腈（50:50, v/v)沉淀蛋白、正己烷萃取,以Phenomenex Kinetex F5色谱柱为分离柱,2.5 mmol/L甲酸铵-0.1%甲酸水溶液和甲醇为流动相,梯度洗脱,电喷雾电离（ESI+ ）、多反应监测（MRM）模式下检测,同位素内标法定量。结果 血清中6种脂溶性维生素线性范围内线性关系良好,相关系数 r >0.995;6种脂溶性维生素的检测限为0.20~1.25 ng/ml,定量限为0.39~3.88 ng/ml;加标回收率为86.6%~107.7%,日内精密度<9.6%,日间精密度<9.3%。NIST标准参照品SRM 968f验证方法准确度,结果偏差均在5%以内。结论 本方法准确度高、重现性好、用血量少,适于婴幼儿等采血困难者微量血样中多种脂溶性维生素的同时快速检测。     

膝关节置换术后骨密度变化的研究进展

目的总结膝关节置换术后骨密度的变化及其诊断方式、影响因素和药物防治研究进展。方法查阅近年国内外有关文献，对骨密度评估测量方式的优缺点、膝关节置换术后骨密度的变化趋势及其影响因素，以及药物防治疗效差异进行总结。结果膝关节置换术后全身骨密度及假体周围平均骨密度总体呈下降趋势，与检测时患者体位、年龄、体质量、日常活动、假体固定方式、假体设计以及假体材料等因素密切相关。狄诺塞麦、双膦酸盐和特立帕肽等药物能够减少膝关节置换术后骨密度降低程度。结论膝关节置换术后骨密度呈下降趋势，但发生机制尚不明确，与多种因素相关。目前，抑制骨吸收药物对于膝关节置换术后骨密度降低有一定效果，但远期疗效有待进一步探究。     

古草生机汤对H22荷瘤小鼠体内抑瘤及免疫调节作用的初步研究

目的：探究古草生机汤对H22荷瘤小鼠体内实体瘤的抑瘤功效和对机体的免疫调节作用机制。方法：本研究采用H22实体瘤动物模型,随机分为空白组、模型组、阳性药组、古草生机汤低、高剂量组,灌胃给药7 d,计算各组小鼠的体质量增长率、肿瘤抑制率、胸腺及脾指数,小鼠实体瘤病理切片苏木精-伊红（HE）染色观察瘤体组织和细胞形态,酶联免疫吸附试验法检测小鼠血清中γ干扰素（IFN-γ）、肿瘤坏死因子-α(TNF-α)、白细胞介素-2（IL-2）、Fas、Fas配体、天门冬氨酸氨基转移酶（AST）、丙氨酸氨基转移酶（ALT）的含量,实时荧光定量PCR测量小鼠瘤组织中Bax和Bcl-2mRNA的相对表达量。结果：古草生机汤有促进H22荷瘤小鼠体质量增长、抑制体内实体瘤增长和促进肿瘤凋亡坏死的作用,可提高小鼠的胸腺指数同时降低脾脏指数,可显著提高小鼠血清中IFN-γ、TNF-α、IL-2的含量并降低Fas、Fas配体、AST、ALT的含量（均P<0.01）,能够上调小鼠瘤组织中Bax mRNA的表达并下调Bcl-2mRNA的表达。结论：古草生机汤具有明显的体内抗肝肿瘤药效,在抑制肿瘤生长、促进肿瘤细胞凋亡、调节机体免疫方面有一定作用。