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71.
新生儿重组酵母乙肝疫苗接种免疫的研究   总被引:1,自引:0,他引:1  
目的:探讨重组酵母乙肝疫苗新生儿接种后抗体应答持续时间,强化复种的必要性。方法:常规对新生儿0d(出生后当天)、1月、6月接种重组酵母乙肝疫苗后检测抗体应答情况,再随机分两组,一组为强化组,一组为常规组,并随访其5年的抗体应答情况。结果:新生儿常规接种法,于12个月后有一明显抗体应答下降期(0d、1月、6月、12月),强化组乙肝表面抗体形成率高,持续时间均高于常规接种法。结论:新生儿乙肝疫苗0d、1月、6月、12月接种法有较好的远期保护效果,对现有的0d、1月、6月新生儿乙肝疫苗常规接种法,有强化接种的必要。  相似文献   
72.
目的 了解湘西自治州重点人群性病患消长趋势,为性病防治工作提供科学依据。方法 从1995年起,采用统一的表格,每年对湘西州劳教所新入教人员进行一次法定性病监测。结果 三种法定性病平均患病率为14.64%(4.96~26.7%),以1995年最低,1997年最高,8年未发现HIV/AIDS,患病率以20~39岁的性跃期人群为最高,汉族患病率高于其它民族;化程度越高,患病率越低。结论 男性劳教人员作为性病患病的高危人群,是哨点监测理想的目标人群。  相似文献   
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74.
OBJECTIVE: To investigate the feasibility of intracoronary application of endothelial progenitor cells and the subsequent distribution within the heart. METHODS: Endothelial progenitors cells (EPCs) cultured from rat bone marrow were identified by double-positive staining with Dil-Ac-LDL and BS1-lectin. Twenty-four hours before cell transplantation, EPCs were labeled with 5-bromo-2'-deoxyuridine (BrdU). Cells (5 x 10(5) in 250-microl medium) were injected into healthy rats, either as intracoronary application (n=11) or as intramyocardial injection (n = 6). At 15 min or 3 days posttransplantation, hearts as well as other organs (lung, liver, kidney, and spleen) were collected and processed for subsequent BrdU immunohistochemistry. The number of BrdU-positive cells per tissue area was counted. RESULTS: Compared to intramyocardial injection, intracoronary administration resulted in more than twice as much positive cells in the heart (P < .05), with no local differences within the heart. Whereas after 15 min, EPCs were equally distributed in all examined organs (except for the spleen), cells that were still present after 3 days, approximately 10%, were selectively restricted to the heart. CONCLUSIONS: Our data indicate that the intracoronary application provides a promising technique for EPC transplantation in the rat heart.  相似文献   
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76.
Frog heart relaxation was analyzed under voltage clamp conditions as the tension decay observed after the membrane potential had been returned to its resting value. The tension decayed exponentially with a time constant of 188±3.8 ms SEM. The relaxation rate decreased with the external Na concentration. It fell to about one tenth in a Na-free solution. Increasing the intracellular Na-content by an application of veratrine also decreased the relaxation rate. Thus relaxation seems dependent on the Na gradient. The relaxation rate decreased within one second upon switching from a high to a low Na-containing solution. The relaxation rate reached a minimum before rising slightly to a new steady state value. This rebound may reflect the partial recovery of the Na gradient since a fast variation in [Na]i follows alteration of [Na]o. Mn and La ions also slowed relaxation. In a Na-free solution, adrenaline accelerated tension decay, an effect not noticeable in frog heart contained in Ringer solution. Other cAMP-promoting agents, such as dibutyryl-cAMP and aminophylline, also increased relaxation rate.It is concluded that in frog myocardium, part of the decrease of the intracellular Ca2+-concentration which occurs during each cardiac cycle could be dependent on a Na–Ca exchange mechanism. The relative importance of this mechanism, versus internal Ca sequestration, in the relaxation of tension may well be greater in contractile tissues whose cells have a large surface/volume ratio.  相似文献   
77.
Apoptosis, the programmed death of cells, plays a distinct role in the etiopathogenesis of Multiple sclerosis (MS), a common disease of the central nervous system with complex genetic background. Yet, it is not clear whether the impact of apoptosis is due to altered apoptotic behaviour caused by variations of apoptosis-related genes. Instead, apoptosis in MS may also represent a secondary response to cellular stress during acute inflammation in the central nervous system. Here, we screened 202 apoptosis-related genes for association by genotyping 202 microsatellite markers in initially 160 MS patients and 160 controls, both divided in 4 sets of pooled DNA samples, respectively. When applying Bonferroni correction, no significant differences in allele frequencies were detected between MS patients and controls. Nevertheless, we chose 7 markers for retyping in individual DNA samples, thereby eliminating 6 markers from the list of candidates. The remaining candidate, the ERBB3 gene microsatellite, was genotyped in additional 245 MS patients and controls. No association of the ERBB3 marker with the disease was detected in these additional cohorts. In consequence, we did not find further evidence for apoptosis-related genes as predisposition factors in MS.  相似文献   
78.
The effectiveness of galactomannan detection with the Platelia test was evaluated in a prospective study of 3,327 sera from 807 patients. The specificity was 99.6% (748 of 751 cases). For the groups of patients with proven and probable invasive aspergillosis, the sensitivity was 50.0% (17 of 34 cases). The disappointing sensitivity associated with the presence of rare false-positive cases underlines the limits of this test.  相似文献   
79.
某些甲状腺疾病时血清可溶性白细胞介素2受体(sIL-2R)水平及其与游离甲状腺素(FT_4)、游离三碘甲腺原氨酸(FT_3)和促甲状腺素(TSH)水平的相关性比较。结果发现甲状腺机能亢进症(甲亢)未治疗组(A)及甲亢未治疗伴突眼组(D)血清sIL-2R明显升高;甲状腺机能减退症(甲减)经治疗甲状腺功能灭常组(G)sIL-2R明显高于甲减未治疗组(F);10例毒性弥漫性甲状腺肿(Graves病)患者经抗甲状腺药物治疗后sIL-2R明显降低;Graves病及甲减患者血清sIL-2R均与FT_3呈正相关。提示除自身免疫外,甲状腺素水平也是甲状腺疾病患者血清sIL-2R水平的重要调节因素。  相似文献   
80.
To determine functional differences between the two splice variants of PPARgamma (gamma1 and gamma2), we sought to selectively repress gamma2 expression by targeting engineered zinc finger repressor proteins (ZFPs) to the gamma2-specific promoter, P2. In 3T3-L1 cells, expression of ZFP55 resulted in >50% reduction in gamma2 expression but had no effect on gamma1, whereas adipogenesis was similarly reduced by 50%. However, ZFP54 virtually abolished both gamma2 and gamma1 expression, and completely blocked adipogenesis. Overexpression of exogenous gamma2 in the ZFP54-expressing cells completely restored adipogenesis, whereas overexpression of gamma1 had no effect. This finding clearly identifies a unique role for the PPARgamma2 isoform.  相似文献   
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