脑缺血后TLR4作用与小胶质细胞的激活

脑缺血性损伤早期小胶质细胞即被激活。激活的小胶质细胞既有细胞毒性又有神经营养作用。小胶质细胞行使免疫功能的信号转导受体之一是TLR4（toll-like receptor 4）。TLR4在脑内主要表达在小胶质细胞，是一种模式识别受体（pattern recognition receptor，PRR）, 识别一些外源性和内源性的配体。最近的研究表明，TLR4信号通路在脑缺血再灌注损伤中起重要作用。TLR4通过激活小胶质细胞，大量表达炎症因子，加重脑缺血性损伤。     

心电信号预处理与心电信号分析

本文介绍了在一种便携式心电监护仪器中是如何对心电数据进行预处理和智能分析的．为了适应便携式仪器的特征，我们在心电信号预处理中采用了FFT滤波和滑动平均滤波的方法去除各种干扰并使图像得以平滑，同时采用了差分阈值法提取特征点，考虑到监护仪器的实用性，在心电信号分析阶段，我们采用了分析特征间期异常情况的方法来替代对病症的智能诊断功能。     

An ER export signal accelerates the surface expression of shal potassium channels in pyloric neurons of the lobster stomatogastric ganglion

The shal gene encoding the transient potassium current, I _A, plays important roles in shaping the firing properties of neurons in the pyloric network in the stomatogastric ganglion (STG) of the spiny lobster, Panulirus interruptus. However, when we overexpressed the shal protein in pyloric dilator (PD) neurons, the effect of increased I _A was compensated by a parallel upregulation of the hyperpolarization activated inward current (I _h). In an attempt to temporally separate the overexpression of shal from the compensatory up-regulation of I _h channels, we inserted an endoplasmic reticulum (ER) export signal sequence, FCYENE, into the shal gene. This signal sequence accelerated the surface expression of shal protein in Xenopus oocytes and PD neurons. However, the accelerated expression of shal still did not alter the firing properties of the injected neuron, suggesting that the compensatory upregulation of I _h occurs simultaneously with the upregulation of I _A.     

钙调神经磷酸酶参与心衰患者心肌重构的信号转导

目的：探讨血管紧张素Ⅱ(Ang Ⅱ)介导的钙调神经磷酸酶（CaN）信号通路参与心力衰竭（CHF）患者心肌重塑的机制。方法:选择因瓣膜性心脏病接受二尖瓣置换术的CHF病人39例，正常对照38例(其中8例来自意外伤亡的器官捐献者)。彩色多普勒超声心动图仪检测心脏扩大和心功能参数。放免法检测血浆及心肌组织Ang Ⅱ浓度，免疫沉淀法测心肌组织CaN、活化T细胞核因子(NFAT₃）、锌指转录因子(GATA₄)磷酸化及蛋白表达，RT-PCR检测肌球蛋白重链（β-MHC）mRNA表达。结果:AngⅡ分别与心脏扩大参数呈显著正相关，而与心功能参数呈显著负相关。CHF患者心肌组织CaN蛋白表达、CaN磷酸化、GATA^₄蛋白表达及β-MHC mRNA表达明显高于对照组，随心功能恶化其表达逐渐增加；NFAT₃磷酸化随心功能恶化而减弱。结论：肾素血管紧张素系统（RAS）激活的CaN信号通路在CHF患者心肌重构机制中可能起重要作用。     

p38应急信号通路参与一氧化氮诱导PC12细胞死亡

目的:探讨一氧化氮诱导PC12细胞死亡的信号转导途径。方法:将亚硝基铁氰化钠(sodiumnitroprusside,SNP)、caspase-3拮抗剂(caspase-3inhibitorⅡ)加SNP或p38拮抗剂(SB203580)加SNP与传代培养的PC12细胞一起孵育,观测细胞的存活率和caspase-3的活性;用MTT法测细胞存活率,caspase-3检测试剂盒测caspase-3活性。结果:SNP以浓度和时间依赖性方式诱导PC12细胞死亡,并增加caspase-3的活性;caspase-3拮抗剂Ⅱ和p38拮抗剂均明显减少细胞死亡且p38拮抗剂明显降低caspase-3的活性。结论:一氧化氮可能通过激活p38、caspase-3信号分子诱导PC12细胞死亡。     

A dual participation of ZAP-70 and scr protein tyrosine kinases is required for TCR-induced tyrosine phosphorylation of Sam68 in Jurkat T cells

Sam68 has been initially described as a substrate of src kinases during mitosis in fibroblasts. Recent evidence suggests that in T lymphocytes Sam68 may act as an adaptor protein and participate in the early biochemical cascade triggered after CD3 stimulation. A direct interaction between Sam68 and the two src kinases involved in T cell activation, p59^fyn and p56^lck, as well as a partnership of Sam68 with various key downstream signaling molecules, like phospholipase Cγ-1 and Grb2, has been shown. In this study we analyze the contribution of p56^lck, as well as the role of ZAP-70, the second class of protein tyrosine kinase involved in T cell activation, in Sam68 tyrosine phosphorylation in the human Jurkat T cell line. Using the src inhibitor PP1 [4-amino-5-(4-methylphenyl)7-(t-butyl) pyrazolo [3,4-d] pyrymidine] and cell variants with defective expression of p56^lck or expressing a dominant negative form of ZAP-70, we demonstrate that, while both p56^lck and ZAP-70 are dispensable for the low constitutive phosphorylation of Sam68 observed in Jurkat cells, a cooperation between the two kinases is required to increase its rapid phosphorylation observed in vivo after CD3 stimulation. We also show that recombinant forms of both p56^lck and ZAP-70 phosphorylate Sam68 in vitro. However, using CD2 stimulated cells, we observe that p56^lck activation by itself does not induce Sam68 tyrosine phosphorylation. We conclude that p59^lck and p56^lck differently participate in regulating the phosphorylation state of Sam68 in T cells and that ZAP-70 may contribute to Sam68 tyrosine phosphorylation and to the specific recruitment of this molecule after CD3 stimulation.     

Nature of Rec+ revertants isolated from Escherichia coli K-12 cultures with recA- mutations

The nature of Rec⁺ revertants isolated previously from cultures of recombinationally defective strainEscherichia coli K-12 AB 2463 recA13 was studied. With the aid of phage P1 vira the chromosome region of the recA gene in cells of strain JC2915F^- were transduced, after which the recombination capacity of the transductants was determined by crossing with JC158Hfr cells and their resistance to ultraviolet radiation was established. Sensitivity of the transductants to suppressor phages was determined. The Rec⁺ revertants were shown to differ with respect to the recA gene. In some Rec⁺ revertants the Rec⁺ phenotype appeared as the result of a back mutation in this gene from rec^- to rec⁺, whereas in other revertants the Rec⁺ phenotype was due to indirect suppression.Department of Biology and General Genetics, Patrice Lumumba Peoples' Friendship University, Moscow. (Presented by Academician of the Academy of Medical Sciences of the USSR V. M. Zhdanov.) Translated from Byulleten' Éksperimental'noi Biologii i Meditsiny, Vol. 82, No. 12, pp. 1487–1488, December, 1976.     

Blockade of CD40-CD40 ligand pathway induces tolerance in murine contact hypersensitivity

Interactions between CD40 on antigen-presenting cells and its ligand (CD40L) on T cells has been implicated in T cell-mediated immune responses. Previously, we have shown that contact hypersensitivity (CHS), a cell-mediated cutaneous immune response in reaction to haptens, could be subclassified based on whether the hapten primed for Th1 or Th2 cytokines in cells isolated from draining lymph nodes. We also found that tolerance to a Th2-priming hapten could be induced only by simultane blockade of the CD40-CD40L and B7-CD28 at the time of sensitization. Here we demonstrate that blockade of CD40-CD40L signaling alone induces long-lasting unresponsiveness to the Th1 hapten 2,4-dinitrofluorobenzene (DNFB), and inhibits antigen-specific T cell proliferation in vitro. We find that CD40-CD40L signaling is required in the sensitization but not elicitation phase of DNFB-induced CHS, as treatment of mice with anti-CD40L monoclonal antibody (mAb) does not affect the response to hapten challenge in previously sensitized and untreated animals. Examination of cytokine production shows that anti-CD40L mAb decreases interferon-γ production by draining lymph node cells from DNFB-sensitized mice, and reciprocally increases interleukin (IL)-4 production. Consistent with this Th1 to Th2 immune deviation, anti-CD40L mAb prevents the induction of IL-12 mRNA in regional lymph nodes, an event which is normally seen within 12 h following hapten sensitization. In contrast, suppression of CHS by CTLA4Ig decreased the production of all cytokines by draining lymph node cells. Together, these data show that blockade of the CD40-CD40L pathway by itself is sufficient to induce tolerance to DNFB-induced CHS, and that this is associated with blockade of IL-12 induction and Th1 to Th2 immune deviation.     

Ampullary electroreceptors in catfish (Teleostei): temperature dependence of stimulus transduction

The response properties of ampullary electroreceptors have been studied in the catfish Ictalurus nebulosus at skin temperatures between 5 and 35 °C. A unimodal relationship between spontaneous activity and temperature was obtained. Mean (±SEM) peak discharge rate was 57.3 ±1.8 impulses s^–1 at 25 ° C; the receptors were active at 5 °C (15.0 impulses s^–1) and at 35 °C (31.5 impulses s^–1). There were no dynamic responses to temperature changes in either the warming or cooling direction. The shape of the frequency characteristic depended on temperature: the peak of the gain curve shifted to low frequencies at low temperatures. There was a concomitant change of the phase characteristic: the intersection at zero degree phase angle shifted to higher frequencies with an increase of temperature, thus increasing the lead at lower frequencies and decreasing the lag at higher frequencies. Latency after combined excitatory and inhibitory impulse stimulation was temperature dependent, ranging from 16.4 ms (5 °C) to 5.6 ms (35 °C). Application of the specific calcium channel blocker menthol (0.2 mM) suppressed spontaneous activity, the effect becoming more prominent at higher temperatures. Sensitivity to sinusoidal electrical stimulation was also impaired, but to a lesser degree and mainly at lower temperatures. We conclude that the filter properties of the receptor organ can be modelled by a band-pass filter in series with a latency, both of which are temperature dependent. These filter properties might be partially based on the activation kinetics of the tranduction channels.     

Methods for non-invasive detection of ventricular late potentials--a comparative multicenter study

To evaluate the methodological problems of the non-invasive registration of late potentials the results obtained with four different averaging devices in the same 109 patients were compared. The high-resolution ECG was obtained from the body surface, high-gain amplified and filtered. With the averaging technique, the improved signal-to-noise ratio was able to detect low-amplitude cardiac activity. The incidence of late potentials detected with the four averaging systems, whose characteristics are described, ranged between 12% and 21%. Corresponding positive results were obtained in 5.5%, corresponding negative results in 68.8%. The reasons for differing results were mainly due to differences in visual or automatic interpretation of the registered fractionated electrical cardiac activity. Additionally, the determination of the end of QRS using the QRS width, obtained from reference leads, may influence the specificity of the methods.