Interferences with semen detection by an immunoassay for a seminal vesicle-specific antigen

A commercial enzyme-linked immunosorbent assay (ELISA), the SEMA assay, for a seminal vesicle-specific antigen (SVSA) provides highly sensitive detection of semen. Here we show marked interference of proteins such as albumin, serum proteins, or mucin with the assay. This would substantially decrease the sensitivity for detecting semen mixed with other biological fluids such as blood or vaginal secretions.     

An enzyme-linked immunosorbent assay (ELISA) for human semen identification based on a biotinylated monoclonal antibody to a seminal vesicle-specific antigen

Monoclonal antibody mouse antihuman semen-5 (MHS-5) (immunoglobulin G1 [IgG1]) was biotinylated using N-biotinyl-w-aminocaproic acid-N-hydroxysuccinimide ester. This monoclonal antibody-biotin conjugate recognized low molecular weight peptide bands between 10.5 and 20 kilodaltons on immunoblots of liquefied semen. Immunodominant peptides had molecular weights of 10.5, 11.5, and 13.5 kilodaltons. An enzyme-linked immunosorbent assay (ELISA) developed with the biotinylated-MAb and streptavidin peroxidase demonstrated sensitivity curves with lower limits of 10 ng of seminal fluid protein per microtiter well using 50 ng per well of monoclonal antibody-biotin conjugate. Cross-reactivity studies on a panel of human biological fluids and tissues demonstrated no cross-reactivity or false positives using the monoclonal antibody-biotin conjugate. The sensitivity of the monoclonal antibody-biotin ELISA was compared to ELISA based upon a polyclonal secondary antibody-peroxidase conjugate. These findings indicate that this ELISA assay, based on a biotinylated monoclonal antibody to a seminal vesicle-specific antigen, may be useful for semen identification.     

Evaluation of prostate-specific antigen (PSA) membrane test assays for the forensic identification of seminal fluid.

Prostate specific antigen (PSA, also known as p30), a glycoprotein produced by the prostatic gland and secreted into seminal plasma, is a marker used for demonstrating the presence of seminal fluid. Methods for the detection of PSA include Ouchterlony double diffusion, crossover electrophoresis, rocket immuno-electrophoresis, radial immunodiffusion, and ELISA. The extremely sensitive ELISA technique can detect PSA in concentrations as low as approximately 4 ng/mL. However, all these techniques are cumbersome and time consuming to perform in forensic laboratories, especially when only a few samples per week are processed. Various membrane tests are currently used in clinical settings to screen a patient's serum for the presence of PSA at levels greater than 4 ng/mL. In this study we evaluated three immunochromatographic PSA membrane tests by analyzing semen stains stored at room temperature for up to 30 years, post-coital vaginal swabs taken at different time after intercourse, semen-free vaginal swabs, and various female and male body fluids, including urine. The data demonstrate that PSA membrane test assays offer the same sensitivity as ELISA-based tests and provide a rapid approach for the forensic identification of seminal fluid. Furthermore, when the supernatant from a DNA extraction is used for the assay, there is essentially no DNA consumption for determining the presence of PSA in a forensic sample.     

闭合性脑损伤后血清和海马的蛋白质表达

目的 研究大鼠脑损伤后血清和海马中蛋白质表达的差异.方法 用雄性SD大鼠制造脑损伤模型,应用弱阳离子交换(WCX2)芯片和铜离子结合(IMAC-Cu)芯片结合表面增强激光解析电离飞行时间质谱技术,分析大鼠闭合性脑损伤后不同时间血清和海马中蛋白质表达谱的变化.结果 WCX2芯片在血清和海马样本中分别捕获436个和364个...     

溺死大鼠肺组织水通道蛋白1的表达

目的检测生前溺死与死后抛尸的肺组织水通道蛋白的表达。方法取2种死亡方式条件下大鼠肺组织,用免疫组织化学方法检测肺组织中水通道蛋白1表达的分布特征。结果两种死亡条件下肺泡间质和支气管周围的毛细血管内皮及肺泡上皮均有AQP1的阳性表达,但积分光密度值(intergratedopticaldensity,IOD)值有显著性差别。结论AQP1在大鼠两种溺死条件下表达差别有统计学意义。     

The use of scanning electron microscopy in the examination of seminal stains

Samples of human seminal stains on fabrics, paper and wood were observed with a scanning electron microscope (S.E.M). It seems a reliable, rapid and simple technique for the routine examination of seminal stains.     

过敏性休克急死豚鼠血清和肺组织内IgE的变化及法医学意义

目的研究过敏性休克急死豚鼠死后在4℃冷藏条件下血清IgE含量和肺组织内IgE的免疫表达随死后不同时间的变化,探讨过敏性休克急死的法医学鉴定的客观诊断指标。方法采用多人混合血清注射建立过敏性休克急死的动物模型。豚鼠40只,随机分为对照组和实验组,实验组又分为死后0、12、24和48h组,每组8只。采用酶联免疫吸附试验测定豚鼠血清IgE含量,采用免疫组化ABC法对豚鼠肺组织IgE进行免疫组化染色。结果实验组与对照组豚鼠血清IgE含量相比较有显著性差异(P<0.001);死后0、12、24和48组血清IgE含量相比较无显著性差异(P>0.05)。实验组豚鼠肺组织IgE有阳性表达,对照组豚鼠无IgE表达。结论过敏性休克急死豚鼠血清IgE含量显著升高;在4℃下冷藏,死后48h内血清IgE含量和肺组织中IgE无明显变化。本结果可为过敏性休克急死的法医学鉴定提供客观的诊断依据。     

The detection of protein p30 in seminal stains by means of thin-layer immunoassay

The detection of p30 by means of an indirect thin-layer immunoassay (TIA) is described. Extracts from 20 samples can be analyzed in approximately 2 h with a detection limit of approximately 50 ng. The p30 protein was detected in seminal stains which had been stored at room temperature for six months and at 130 degrees C for 4 h. Blood, saliva, urine, perspiration, and tears did not interfere with the method. The reliability of the method was demonstrated in a blind study.     

Defects in medical care delivery to patients with lung and breast cancer undergoing radiotherapy

Patients aged 55 and 63 years received extracorporeal 30 and 40 Gy gamma-therapy for lung cancer, respectively. Two and 60 days after irradiation, respectively, the patients developed arrosive pulmonary hemorrhage with lethal outcomes. Forensic medical examination in both cases has detected acute radiation pneumonitis with impairment of pulmonary artery endothelium that provoked hemorrhage. The literature review covers acute and chronic lesions of the lungs in radiotherapy of lung and breast tumors.     

Evaluation of three rapid detection methods for the forensic identification of seminal fluid in rape cases

We sought to discover whether spermatozoa concentration and the delay between ejaculation and test influence the results of seminal fluid fast detection tests. Two hundred and twenty-seven anonymous samples divided into four groups (normospermia, oligospermia, azoospermia, and controls) after a semen analysis were subjected to three fast detection semen tests: Diff-Quick fast coloration, Phosphatesmo Km Paper for acid phosphatases (AP) detection, and PSA-Check 1 for prostate specific antigen (PSA) detection. The study was performed at three time points (0, 48, and 72 h). Unlike cytology, results obtained with AP and PSA were not influenced by spermatozoa concentration. PSA detection results remained constant up to 72 h and were more reliable after 48 h than those obtained by AP detection.     

Detection of amphetamine in bloodstains,semen, seminal stains,saliva, and saliva stains

Low nanogram quantities of amphetamine were detected in 100μl samples of dried bloodstains using radioimmunoassay. Saliva, saliva stains, semen, and seminal stains also contained measurable quantities of the drug.     

四类遗传标记的检测用于混合精斑的个人识别

目的探讨综合应用常染色体STR与Y-STR、X-STR、mtDNA高变区Ⅰ序列检测四类遗传标记,提高两男性混合精液样品的个人识别率。方法使用商品化试剂盒检测混合精液样品的常染色体与X、Y染色体STR,应用单链构象多态性(single strand conformation polymorphism,SSCP)法分离两男性混合精液样品的线粒体DNA(mitochondrial DNA,mtDNA)高变区Ⅰ序列,并进行序列分析。结果混合精液样品比例超过1:10(高组分所占比例继续增加而低组分所占比例继续减少)时可以确定高拷贝者的全部四类遗传标记系统的分型。比例接近时,通过与嫌疑人检测结果的比较可获得排除或基本认定的意见。结论四类遗传标记系统的联合检测有助于提高两男性混合精液样品的个人识别率。     

DCM猝死与晚期DCM心肌Cx43表达的比较

目的观察和探讨扩张型心肌病(DCM)猝死与晚期DCM心肌中心肌连接蛋白(connexin,Cx)43表达差异及其意义。方法收集13例DCM猝死者心脏(A组)和5例晚期DCM患者行心脏移植手术切除的心脏(B组),运用免疫组化染色和图像分析技术,检测心肌Cx43阳性表达产物的平均光密度(OD)值和面积(S)值,比较两组间和左右心室间的差异。结果 Cx43阳性表达在A组明显减少,分布不均;在B组表达清晰,主要位于闰盘处。A组与B组心肌Cx43的S值之间的差异有统计学意义(P0.01),而各组左、右心室肌间相比,差异无统计学意义(P0.05);心肌Cx43的OD值,在A组与B组之间,以及各组左、右心室肌间差异均无统计学意义(P0.05)。结论 DCM猝死心肌Cx43表达较晚期DCM心肌明显减少,这种变化可能与DCM患者因心律失常发生猝死有关。