C6-polymorphism of the sixth component of complement: application to paternity cases (author's transl)]

The results of a study of the polymorphism of the sixth component of human complement by means of isoelectric focusing in polyacrylamide gels with subsequent C-dependent lysis in an agarose overlay containing C6 deficient rabbit serum are reported. The allele frequencies obtained (C6A = 0.613, C6B = 0.379, C6R = 0.008) are in good agreement with those previously published. The mode of inheritance in 47 families with 173 offspring as well as 26 mother-child combinations is in agreement with a formal genetical model: "C6A, C6B, C6A1 and C6B1 at an autosomal locus". The inclusion of this system into a blood group expertise in Germany can be recommended.     

Forensic application and polymorphism of the human lysosomal α-fucosidase (E.C.3.2.1.51)

Blood samples from 468 unrelated persons in Northrhine-Westphalia (F.R.G.) were tested in order to determine the frequency of the two common alleles at the FUCA-locus. In our series, the gene frequencies could be calculated as follows: FUCA¹:0.7447; FUCA²:0.2553. The plausibility to exclude non fathers from paternity is 15.4%.     

The typing of group-specific component (Gc protein) in human blood stains

It is known that the typing of group-specific component (Gc protein) in human blood stains is difficult since Gc protein of the extracts of blood stains migrates more anodally to the α₁-globulin region in agar-gel immunoelectrophoresis, while Gc protein in liquid blood normally migrates to the α₂-globulin region. We have reported that the Gc protein found in the α₁-region is the result of binding of actin to Gc protein (Shinomiya, K., Kimura, H., Yoshida, K., and Shinomiya, T., J. Biochem., 92 (1982) 1163–1171, which renders it difficult to determine the Gc-phenotypes in the blood stains. On the basis of the above findings, we developed the method of phenotyping the Gc protein of human blood stains by agar-gel immunoelectrophoresis. Since the binding activity of actin to Gc protein is lost after treatment with a high concentration of guanidine HCl, the extracts of blood stains were treated with 4 M guanidine HCl to dissociate Gc protein and actin and then dialyzed to remove guanidine HCl. By this method we are able to determine the phenotypes of Gc protein in blood stains. The method we have developed is a useful tool in the forensic laboratory.     

用等位基因特异扩增技术检测人类补体第八成份C8A DNA多态性的研究

建立补体第八成份蛋白质多态性的DNA检测方法。根据导致C8A多态性的DNA点突变核苷酸差异 ,建立一个检测C8A基因型的特异性扩增方法。采用该法 ,对 10 0份血样本进行检测 ,并同时用传统的检测C8A蛋白质多态性的SDS 凝胶电泳方法进行对照检测 ,结果显示新建立的C8A多态性PCR分型方法不仅快速、灵敏、稳定 ,而且分型结果清晰 ,容易判读 ,适用于法医学中多种检材的C8A多态性分型     

Genetic polymorphism of human C1R subcomponent of the first complement component in the Japanese population

Genetic polymorphism of the C1R subcomponent of human complement component C1 has been investigated in neuraminidase treated EDTA plasma samples of 440 healthy Japanese individuals living in Tokyo by means of thin-layer polyacrylamide gel isoelectric focusing (PAGIEF) at pH 3.5-9.5 in the presence of 8.0 M urea followed by an electroblotting with enzyme immunoassay. Three common and three rare alleles were detected in the Japanese population. Of these, two common alleles were identical to C1R*1 and C1R*2 and other new alleles were tentatively designated C1R*3, C1R*4, C1R*5 and C1R*6, respectively. The results of the family studies suggested that the genetic model for C1R polymorphism assumed autosomal codominant Mendelian inheritance. The allele frequencies were estimated as C1R*1 = 0.4216, C1R*2 = 0.3602, C1R*3 = 0.2068, C1R*4 = 0.0091 and C1R*R(C1R*5 and C1R*6) = 0.0023, respectively. The distribution of allotypes fitted the Hardy-Weinberg equilibrium. The C1R system provides a useful genetic marker for human genetics, anthropologic studies and forensic science.     

Polymorphism of the third component (C3) of complement and of Transferrin (Tf) in Belgium.

The phenotypes of C3 and of Tf were determined in 818 and 576, respectively, unrelated individuals living in Liege. The gene frequencies observed are: (formula: see text) The application to disputed paternity cases and to the study of twins is discussed.     

Forensic application of the polymorphism of coagulation factor XIIIB

Gene frequencies of coagulation factor XIIIB polymorphism were determined in a random population sample of east Westphalia (n = 417). Furthermore, mendelian inheritance of alleles was examined in 60 families. Determinations were made after treatment of serum samples with neuraminidase by immunofixation on agarose gels. All six phenotypes were observed in our population sample. The gene frequencies were: FXIIIB1 = 0.71, FXIIIB2 = 0.11, FXIIIB3 = 0.18. The family data confirm the hypothesis of autosomal inheritance of three common alleles and disprove the two-allele model of Kera et al. [5].     

Estimation of postmortem interval based on the third component of complement (C3) cleavage

To estimate postmortem interval (PMI), the spontaneous conversion of the native third component of complement (C3) to its derived fragments in whole blood was studied by crossed immunoelectrophoresis. C3 cleavages in vitro at different temperatures showed that the incubation of whole blood at a higher temperature led to a faster conversion of beta 1C (native C3) to beta 1A (C3c). In cadaveric blood, we found a significant positive correlation between percentage of C3 cleavage and PMI. From these results, it is possible to estimate PMI from the ratios of C3 cleavage.     

Effects of presumptive test reagents on the ability to obtain restriction fragment length polymorphism (RFLP) patterns from human blood and semen stains.

Some of the commonly used presumptive test reagents for identification of blood and semen could potentially affect the recovery of intact high-molecular-weight deoxyribonucleic acid (DNA) from evidentiary samples. Thus, the capability of performing restriction fragment length polymorphism (RFLP) analysis on evidentiary samples could be compromised. In order to investigate the potential effects of presumptive test reagents on the DNA present in these samples, bloodstains on cotton and glass were exposed directly to luminol, benzidine, phenolphthalein, o-tolidine, and leucomalachite green, while semen stains and vaginal swabs containing semen were exposed directly to bromochloroindolyl phosphate (BCIP) and sodium thymolphthalein monophosphate (STMP) reagents. The yield gels for DNA quality and quantity and RFLP results indicated that bloodstains exposed to luminol, benzidine dissolved in ethanol, and phenolphthalein, as well as semen stains and vaginal swabs exposed to BCIP and STMP yield RFLP patterns consistent with that of the uncontaminated control. Except for the phenolphthalein treatment, the quantity of extractable, high-molecular-weight DNA obtained was comparable with that of untreated stains. Therefore, evidentiary material purposely or inadvertently contaminated with these reagents can be successfully typed. However, stains exposed to benzidine dissolved in glacial acetic acid, leucomalachite green, and o-tolidine failed to yield high-molecular-weight DNA or to produce any RFLP patterns.     

Immunological analysis of human placental lactogen in blood stains and its application to forensic science

Sex determination of blood stains from women who were in the late stages of pregnancy was possible by detecting human placental lactogen (HPL) in them. However, the agglutination time for positive reactions was prolonged as the stains aged.     

Estimation of postmortem interval using kinetic analysis of the third component of complement (C3) cleavage

To estimate postmortem interval (PMI), spontaneous cleavage of the third component of complement (C3) was studied in aged blood and cadaveric blood by crossed immunoelectrophoresis. Using the kinetics of C3 cleavage in vitro described as dC/dt = -kC, where C is the concentration of native C3 at time t and k is a first-order rate constant, Arrhenius' equation, and another equation which assumes a linear drop of body temperature after death, the percentages of C3 cleavage were calculated. There was a significant positive correlation between the calculated percentages and the measured percentages of up to 10% in cadaveric blood. We found that the comparison between the calculated percentage of C3 cleavage for each optional postmortem interval and the measured percentage of up to 10% in cadaveric blood leads to the estimation of PMI. This approach is one step towards the development of an accurate method for determining PMI based on C3 cleavage, that is, on a first-order reaction.     

中国汉族群体人类补体C8A多态性

采用免疫沉淀、SDS-聚丙烯酰胺凝胶电泳 (SDS- PAGE)、被动转印及酶免分析 ,研究了人类补体 C8A等位基因频率在成都地区汉族群体中的分布。 12 1份样本被分为 3种常见型 ,即 C8A- A、C8A- B及 C8A- AB,由两个等位共显性基因 C8A * A及 C8A* B控制 ;同时发现了 2个稀有亚型 ,即 A3亚型及新发现的 Ax亚型。等位基因频率为 C8A* A=0 .5 0 83,C8A* B=0 .4835 ,C8A*稀有型 =0 ,0 0 83。说明 C8A多态性在中国群体中具有良好的分布 ,个人识别率(DP)达到 6 1.14% ,可用于法医学个人识别及亲子鉴定     

C7 typing of blood stains using isoelectric focusing and immunoblotting

By means of isoelectric focusing and immunoblotting C7 types were clearly demonstrated from bloodstains which had been stored at 37 degrees C for up to three weeks, at room temperature for up to six weeks and at 4 degrees C for over ten weeks. The C7 typing is practically useful in medicolegal individualization of unknown bloodstains.     

ABO血型的基因型与法医学应用

ABO血型系统是1901年由Landsteiner首先发现的第一个人类遗传标记.由于ABO血型抗原不仅存在于组织细胞,也存在于体液中,抗原相对稳定,保存较持久,分型已标准化,群体资料丰富,故在法医学上一直有着重要的地位.传统的ABO分型采用血清学方法,但其抗原属糖蛋白易失活,自然界中广泛存在类似的物质,都会影响检验效果.因DNA特殊结构,使得稳定性比蛋白更高,是携带遗传信息的物质,因此,从DNA水平对ABO基因进行分型更能准确地反映个体的差异,尤其是PCR技术对微量检材的检验,ABO血型系统的分子生物学分型法已越来越多地被应用到法医学上[1].     

ABO血型的基因型与法医学应用

ＡＢＯ血型系统是 1 90 1年由Ｌａｎｄｓｔｅｉｎｅｒ首先发现的第一个人类遗传标记。由于ＡＢＯ血型抗原不仅存在于组织细胞 ,也存在于体液中 ,抗原相对稳定 ,保存较持久 ,分型已标准化 ,群体资料丰富 ,故在法医学上一直有着重要的地位。传统的ＡＢＯ分型采用血清学方法 ,但其抗原属糖蛋白易失活 ,自然界中广泛存在类似的物质 ,都会影响检验效果。因ＤＮＡ特殊结构 ,使得稳定性比蛋白更高 ,是携带遗传信息的物质 ,因此 ,从ＤＮＡ水平对ＡＢＯ基因进行分型更能准确地反映个体的差异 ,尤其是ＰＣＲ技术对微量检材的检验 ,ＡＢＯ血型系统的分…