Asynchronous replication timing of imprinted loci is independent of DNA methylation,but consistent with differential subnuclear localization

Genomic imprinting in mammals marks the two parental alleles resulting in differential gene expression. Imprinted loci are characterized by distinct epigenetic modifications such as differential DNA methylation and asynchronous replication timing. To determine the role of DNA methylation in replication timing of imprinted loci, we analyzed replication timing in Dnmt1- and Dnmt3L-deficient embryonic stem (ES) cells, which lack differential DNA methylation and imprinted gene expression. Asynchronous replication is maintained in these ES cells, indicating that asynchronous replication is parent-specific without the requirement for differential DNA methylation. Imprinting centers are required for regional control of imprinted gene expression. Analysis of replication fork movement and three-dimensional RNA and DNA fluorescent in situ hybridization (FISH) analysis of the Igf2-H19 locus in various cell types indicate that the Igf2-H19 imprinting center differentially regulates replication timing of nearby replicons and subnuclear localization. Based on these observations, we suggest a model in which cis elements containing nonmethylation imprints are responsible for the movement of parental imprinted loci to distinct nuclear compartments with different replication characteristics resulting in asynchronous replication timing.     

Defects in regulation of apoptosis in caspase-2-deficient mice

During embryonic development, a large number of cells die naturally to shape the new organism. Members of the caspase family of proteases are essential intracellular death effectors. Herein, we generated caspase-2-deficient mice to evaluate the requirement for this enzyme in various paradigms of apoptosis. Excess numbers of germ cells were endowed in ovaries of mutant mice and the oocytes were found to be resistant to cell death following exposure to chemotherapeutic drugs. Apoptosis mediated by granzyme B and perforin was defective in caspase-2-deficient B lymphoblasts. In contrast, cell death of motor neurons during development was accelerated in caspase-2-deficient mice. In addition, caspase-2-deficient sympathetic neurons underwent apoptosis more effectively than wild-type neurons when deprived of NGF. Thus, caspase-2 acts both as a positive and negative cell death effector, depending upon cell lineage and stage of development.     

Distribution of ferritin in the rat hippocampus after kainate-induced neuronal injury

A gradual increase in iron occurs in the lesioned hippocampus after neuronal injury induced by the excitotoxin kainate, and the present study was carried out to investigate whether this increase in iron might be associated with changes in expression of the iron binding protein, ferritin. An increase in ferritin immunoreactivity was observed in glial cells of the hippocampus, as early as three days after intracerebroventricular injections of kainate. The number of ferritin positive cells peaked four weeks after the kainate injection, and decreased eight and twelve weeks after injection. They were found to be mostly microglia and oligodendrocytes by double immunofluorescence labeling with glial markers. A number of ferritin-labeled endothelial cells were also observed via electron microscopy. The decline in ferritin immunoreactivity four weeks after the injection of kainate is accompanied by an increase in the number of ferric and ferrous iron positive cells in the lesioned tissue. A substantial non-overlap between ferritin and iron-containing cells was observed. In particular, spherical ferric or ferrous iron-laden cells in the degenerating hippocampus were unlabeled for ferritin for long time periods after the kainate injection. An increase in iron, together with a reduced expression of iron binding proteins such as ferritin at long time intervals after kainate lesions, could result in a relative decrease in ferritin-induced ferroxidase activity and the presence of some of the iron in the ferrous form. It is postulated that this may contribute to chronic neuronal injury, following acute kainate-induced neurodegeneration.     

大鼠嗅球和鼻腔嗅粘膜成鞘细胞的形态学研究

目的：观察大鼠嗅神经成鞘细胞在嗅球和嗅粘膜的分布及其形态学结构特征，研究其与中枢神经再生的关系。方法：Luxol固蓝染色、Mallory染色和NGFRp75免疫组织化学染色结合透射电镜观察。结果：在嗅球纤维层的成鞘细胞随神经纤维呈纵向排列，在嗅小球层的成鞘细胞则围绕着嗅小球环行排列。在嗅粘膜的成鞘细胞位于柱状上皮深方，沿基底膜分布。成鞘细胞的胞体为细长梭形，有较长的突起，细胞核呈圆形或椭圆形。在嗅小球周围或嗅粘膜内的成鞘细胞呈NGFRp75免疫反应阳性。在电镜下，嗅球成鞘细胞的纵断面上可见其胞体呈长梭形，细胞核为不规则形，核仁清晰。在胞体的周围有大量的平行神经纤维纵向排列，在放大的横断面上，可见在1个成鞘细胞的细胞核周围有数根神经纤维被胞质包裹在一起。结论：嗅成鞘细胞是一种特殊的胶质细胞，分布于嗅球的纤维层、嗅小球层和嗅粘膜内。嗅神经成鞘细胞的胞体细长，有较长突起，其轴系膜紧密包裹成束的无髓神经纤维。     

睡眠剥夺对词汇背景记忆的影响

目的:探讨睡眠剥夺对于背景记忆的影响。方法:将32名青年被试随机分为四组,分别为剥夺睡眠21小时、45小时、69小时和正常对照组,每组被试8名。正常对照组在早8:00,进行测试;睡眠剥夺组自第一天早7:00进入实验室开始剥夺睡眠,分别在第2天、第3天和第4天凌晨4:00离开实验室。测试为词汇背景记忆测验,通过按键反应,要求被试首先再认是否为旧词,再判断旧词的颜色。结果:除45小时组和69小时组漏过率外,同一组内背景记忆成绩低于再认(P<0.05);剥夺45小时后,与对照组比再认正确率下降(80.26±7.14/92.60±4.31,F=44.213,P=0.000)、漏过率增加(10.44±3.01/3.60±0.58,F=13.667,P=0.000)、反应时延长(0.71±0.25/0.65±0.16,F=22.315,P=0.000);而SD21后,与对照组比背景记忆正确率下降(62.23±7.71/80.10±8.21,F=31.54,P=0.027)、漏过率增加(9.69±3.11/5.83±2.47,F=3.712,P=0.028)、反应时延长(0.93±0.18/0.89±0.24,F=3.093,P=0.027)。结论:睡眠剥夺后再认和背景记忆成绩下降,并随睡眠剥夺时间的延长成绩下降更加明显;睡眠剥夺对背景记忆的影响更大。     

Contribution of BK Ca2+-activated K+ channels to auditory neurotransmission in the Guinea pig cochlea

Large-conductance calcium-activated potassium (BK) channels are known to play a prominent role in the hair cell function of lower vertebrates where these channels determine electrical tuning and regulation of neurotransmitter release. Very little is known, by contrast, about the role of BK channels in the mammalian cochlea. In the current study, we perfused specific toxins in the guinea pig cochlea to characterize the role of BK channels in cochlear neurotransmission. Intracochlear perfusion of charybdotoxin (ChTX) or iberiotoxin (IbTX) reversibly reduced the compound action potential (CAP) of the auditory nerve within minutes. The cochlear microphonics (CM at f1 = 8 kHz and f2 = 9.68 kHz) and their distortion product (DPCM at 2f1-f2) were essentially not affected, suggesting that the BK specific toxins do not alter the active cochlear amplification at the outer hair cells (OHCs). We also tested the effects of these toxins on the whole cell voltage-dependent membrane current of isolated guinea pig inner hair cells (IHCs). ChTX and IbTX reversibly reduced a fast outward current (activating above -40 mV, peaking at 0 mV with a mean activation time constant tau ranging between 0.5 and 1 ms). A similar block of a fast outward current was also observed with the extracellular application of barium ions, which we believe permeate through Ca2+ channels and block BK channels. In situ hybridization of Slo antisense riboprobes and immunocytochemistry demonstrated a strong expression of BK channels in IHCs and spiral ganglion and to a lesser extent in OHCs. Overall, our results clearly revealed the importance of BK channels in mammalian cochlear neurotransmission and demonstrated that at the presynaptic level, fast BK channels are a significant component of the repolarizing current of IHCs.     

长沙地区无偿献血人群隐匿性乙型肝炎病毒感染情况分析

目的 了解长沙地区无偿献血人群隐匿性乙型肝炎病毒感染(occult hepatitis B virus infection,OBI)流行情况,探讨HBV基因型分布特征和S区氨基酸突变的情况。方法 对长沙地区检测结果为HBsAg-/HBV DNA+的无偿献血血液样本进行HBV血清标志物检测,对其中的OBI样本进行HBV病毒载量检测和S区基因扩增,分析血清学标志物抗HBs与病毒载量检出与否的关系,并对扩增产物进行HBV基因分型和突变位点分析。结果 2019年1月—2020年1月长沙地区173 893份无偿献血标本共确认58例OBI样本,OBI流行率为0.033%;共发现7种血清学模式,抗HBc单独阳性最多,占38.98%,所有样本中抗HBc阳性率为89.83%;16例样本能检测出病毒载量,其中14例样本浓度小于100 IU/ml;抗HBs阳性组和阴性组间的病毒载量检出率无统计学差异;75.0%(12/16)样本扩增出S区序列,基因型均为B型,均发生突变,其中11例的HBsAg抗原决定簇及周边主要亲水区域(major hydrophilic region, MHR)发生氨基酸突变。结论 长沙地区无偿献血者中的OBI感染率在全国属于偏低水平;HBV基因型主要是B型,MHR区的氨基酸突变可能是造成OBI的原因,突变有本地特点。     

Engineered NS1 for Sensitive,Specific Zika Virus Diagnosis from Patient Serology

Dengue virus (DENV) and Zika virus (ZIKV) belong to the Flaviviridae family of viruses spread by Aedes aegypti mosquitoes in tropical and subtropical areas. Accurate diagnostic tests to differentiate the 2 infections are necessary for patient management and disease control. Using characterized ZIKV and DENV patient plasma in a blind manner, we validated an ELISA and a rapid immunochromatographic test for ZIKV detection. We engineered the ZIKV nonstructural protein 1 (NS1) for sensitive serologic detection with low cross reactivity against dengue and developed monoclonal antibodies specific for the ZIKV NS1 antigen. As expected, the serologic assays performed better with convalescent than acute plasma samples; the sensitivity ranged from 71% to 88%, depending on the performance of individual tests (IgM/IgG/NS1). Although serologic tests were generally less sensitive with acute samples, our ZIKV NS1 antibodies were able to complement the serologic tests to achieve greater sensitivity for detecting early infections.     

尿胰蛋白酶原—2测定对急性胰腺炎的早期诊断价值

目的 探讨尿胰蛋白酶原－2测定在急腹症中筛选急性胰腺炎的价值。方法 对346例连续就诊的急腹症病人同时测定尿胰蛋白酶原－2及血、尿淀粉酶。结果 41例急性胰腺炎中有38例尿胰蛋白酶原－2阳性,敏感性为92．7％,305例非胰腺炎的急腹症病人有15例假阳性,特异性为95．1％。5例重症急性胰腺炎中尿胰蛋白酶原－2全部阳性。结论 尿胰蛋白酶原－2是急腹症病人筛选急性胰腺炎快而简便的方法,具有较高的特异性和敏感性。     

提高大脑皮质神经元细胞产率以及活性的研究

目的　提高培养大脑皮质神经元的产率以及活性 ,使实验的细胞模型有良好的一致性和可比性。方法　实验分析了大脑皮质神经元培养过程中 ,从选材、取材到分散细胞等一系列步骤中维持细胞活性的内在因素 ,应用细胞形态学指标 ,Trypanblue染色计数分析以及染色观察。结果　每侧大脑皮质得到细胞约 2 .5× 10 6～ 3.0× 10 6个 ,而且种植不同时间 6 ,12 ,48h细胞存活率均在 95 %以上。结论　该法是较好的大脑皮质神经元培养方法。