听源性惊厥易感大鼠室旁核神经元c—fos表达的研究

目的为下丘脑室旁核参与惊厥应答提供形态学资料。方法：以听源性忭厥易大鼠为动物模型，用免疫组织化学ＡＢＣ法显示下丘脑室旁核神经元即早基因ｃ－ｆｏｓ的表达。     

腕关节关节囊内韧带的解剖观察及其创伤学意义

本文描绘了腕关节关节囊内韧带的解剖,其中首次描述了中腕关节的韧带连结,即大、小多角骨,头状骨至舟状骨的韧带和钩骨至三角骨的韧带.本文还论述了与这些韧带连结方式密切相关的腕骨生理运动特点及维持腕关节稳定性的因素.文章还讨论了与腕关节关节囊内韧带有关的腕部创伤学特点.     

接种白血病细胞后小鼠胸腺哺育细胞和免疫器官组织学及组织化学的变化

按种P_(388)白血病患鼠腹水后第3d,小鼠胸腺哺育细胞内的淋巴细胞,酸性磷酸酶和β-葡萄糖苷酸酶阳性率显著增加,而α-醋酸萘酯酶阳性率则下降。胸腺内胸腺细胞上述3种酶细胞化学反应阳性率均显著增加,但胸腺组织结构未见异常。淋巴结和脾脏亦未见异常变化。接种后第9d,患鼠胸腺、淋巴结和脾脏均见白血病细胞浸润、出血和细胞变性等病变,正常结构被破坏,其中淋巴细胞3种酶细胞化学反应的阳性率均显著增加。此时很难从胸腺分离出胸腺哺育细胞。本文结果提示,胸腺和胸腺哺育细胞与这种白血病的发生有密切关系。     

大鼠三角肌前,后部的运动神经元

为了解主动肌与拮抗肌的运动神经元，应用ＨＲＰ逆行追踪技术研究了大鼠三角肌前部、后部的运动神经元。三角肌前部的运动神经元池位于Ｃ４－６脊髓前外侧核背部及其与后外侧核之间。三角肌后部的运动神经元池位于Ｃ４－７脊髓外侧核及其与前外侧核之间。与前池略有重叠。     

延髓后角脑啡肽超微结构定位和非突触部位释放——脑啡肽突触前抑制痛觉传递的形态学基础

阿片肽在后角镇痛的作用机理,被认为是通过突触前抑制一级传入纤维P物质释放的结果,然而始终未获得形态学的证实。鉴于一级传入纤维存在大量阿片受体的事实,曾提出阿片肽突触前抑制可能是通过非突触的轴-轴作用。为了验证这一设想,本文用免疫组化方法,详细观察了大鼠延髓后角浅层亮氨酸脑啡肽(L-ENK)轴突终末的突触结构和胞吐释放。电镜观察显示,延髓后角ENK终末可分为两类,第一类终末除了含圆形小清亮囊泡外,还有较多的大颗粒小泡(一般7个以上),主要分布于Ⅰ层,很少看到此类终末形成突触;第二类终末,一般含较多圆形清亮小泡和少量大颗粒小泡(一般不超过3个),它们分布于Ⅰ层和Ⅱ层,此类终末主要形成轴-树突触和少量的轴-体突触。只见到一例轴-轴突触,其突触后成分为未标记的R型终末,此外还见到ENK阳性树突成为中央终末的突触后成分。在去传入神经条件下,上述各类终末皆可见到ENK阳性大颗粒小泡的胞吐形成,它们皆位于非突触区,而在突触部位可见到清亮小泡胞吐像,上述结果提示后角ENK非突触部位释放可能是哭触后抑制一级传入纤维P物质释放的形态学基础。     

氧分压在体监测仪的研制

作者报道一种稳定性较高的氧分压在体监测，为医学研究、临床诊断提供一种新的可靠的测试方法及设备，具有较大的应用价值。     

Analysis of false negative results in the immunoassay for anti-acetylcholine receptor antibodies in myasthenia gravis

Possible causes for the failure of immunoassays to detect anti-acetylcholine receptor activity in serum from confirmed myasthenia gravis (MG) patients were investigated. A more sensitive assay, using Protein A to trap immune complexes (ARIA), was applied to 65 MG sera which were negative in the usual assay and to 42 normal human sera. Normal and negative MG sera had antibody (Ab) activity in the same range (50-70 pM). Titers present in 70% of normal sera appeared to be specific antireceptor antibodies as defined by tests for antigen specificity. Thus, higher sensitivity assays did not improve discrimination of MG from normals. In a second group of 108 MG sera studied, 48 were negative by the usual assay criteria in a rat acetylcholine receptor immunoassay. Further detailed analysis of this negative group showed that 3/48 had IgG3 antibody not detectable in the test, 14/48 had Ab's recognizing human receptor determinants exclusively, 29/48 had toxin blocking Ab's not determined by immunoassays, and 6/48 were negative in all tests. The results indicate that the exclusive occurrence of toxin-blocking antibodies in MG subjects is a major factor contributing to false negatives in the ARIA test. Estimates of the amount of Ab's with this functionality indicated that they are present in very much smaller amounts than other classes of anti-receptor Ab's. Degree of blocking activity in patient serum showed a fair correlation with severity of disease. Thus, blocking antibodies appear capable of causing all degrees of disease severity in the absence of other types of antireceptor Ab's. The development of a sensitive and quantitative in vitro assay for blocking antibodies combined with the usual immunoassay would be a major improvement for a MG diagnostic test, with greater than 94% positivity predicted.     

Pre-exposure of murine macrophages to lipopolysaccharide inhibits the induction of nitric oxide synthase and reduces leishmanicidal activity

Murine macrophages produce nitric oxide (NO) from L-arginine on stimulation with lipopolysaccharide (LPS), alone or with interferon-γ (IFN-γ). The effect of incubation of macrophages with low concentrations of LPS on NO synthesis on subsequent stimulation was investigated, using a murine macrophage cell line, J774, and peritoneal macrophages from CBA mice. Cells which had been incubated with LPS produced significantly lower amounts of NO, and expressed lower levels of NO synthase activity, following stimulation with IFN-γ and LPS, or with a high concentration of LPS. This effect was not reversed by tumor necrosis factor-α. The ability of CBA macrophages to kill the intracellular parasite Leishmania major was markedly reduced by pre-incubation with LPS. Reduced NO production by macrophages previously exposed to LPS is a manifestation of endotoxin tolerance, and may represent an important means of regulation of NO synthesis and thus a survival mechanism for intracellular parasites.     

A novel negative regulator for IL-1 receptor and Toll-like receptor 4

The Toll-IL-1 receptor (TIR) superfamily, defined by the presence of an intracellular TIR domain, initiates innate immunity via NF-kappaB activation, leading to production of proinflammatory cytokines. ST2 is a member of the TIR family that does not activate NF-kappaB and has been suggested as an important effector molecule of type 2 T helper cell responses. We have recently demonstrated that the membrane bound form of ST2 (ST2L) negatively regulated IL-1RI and TLR4 but not TLR3 signaling by sequestrating the adaptors MyD88 and Mal. In contrast to wild-type mice, ST2 deficient mice failed to develop endotoxin tolerance. Thus, ST2 suppresses IL-1R and TLR4 signaling via MyD88- and Mal-dependent pathways and modulates innate immunity. The results provide a molecular explanation for the role of ST2 in T(H)2 responses since inhibition of TLRs will promote a T(H)2 response and also identify ST2 as a key regulator of endotoxin tolerance.     

Mice lacking the norepinephrine transporter are supersensitive to psychostimulants

The action of norepinephrine (NE) is terminated, in part, by its uptake into presynaptic noradrenergic neurons by the plasma-membrane NE transporter (NET), which is a target for antidepressants and psychostimulants. Disruption of the NET gene in mice prolonged the clearance of NE and elevated extracellular levels of this catecholamine. In a classical test for antidepressant drugs, the NET-deficient (NET-/-) animals behaved like antidepressant-treated wild-type mice. Mutants were hyper-responsive to locomotor stimulation by cocaine or amphetamine. These responses were accompanied by dopamine D2/D3 receptor supersensitivity. Thus altering NET expression significantly modulates midbrain dopaminergic function, an effect that may be an important component of the actions of antidepressants and psychostimulants.