硅珠法在纯化污染检材中的应用

目的改进硅珠法在纯化污染DNA样本中的应用方法。方法对硅珠法中的具体步骤进行改进,直接纯化、浓缩Chelex法获得的不纯DNA,采用IdentifilerTM试剂盒进行复合扩增,产物经ABI3100测序仪分型检测。结果纯化后的DNA获得了满意的DNA分型。结论硅珠法能够有效地去除DNA样本中的污染物,直接用于纯化Chelex-100法提取的DNA。     

4种固相颗粒吸附法提取滤纸血痕DNA效果的比较

目的探讨4种固相颗粒吸附法提取滤纸血痕样本DNA的效果。方法含有1μL静脉血的滤纸血痕180份,分为4组,每组45份。分别采用4种固相颗粒吸附法(DNAIQ~(TM)系统、D盾超敏DNA提取试剂盒、超高效硅珠纯化DNA提取试剂盒和常规的硅珠法)对上述样本进行DNA提取,对比各组DNA溶液的浓度及STR分型检验结果。结果 D盾超敏DNA提取试剂盒[(3.764±1.790)μg/mL]、超高效硅珠纯化DNA提取试剂盒(3.634±1.112)及常规硅珠法(3.350±1.250)提取到DNA溶液的浓度无统计学差异(P0.05),但均高于DNA IQ~(TM)系统(1.864±1.207)(P0.001);D盾超敏DNA提取试剂盒、超高效硅珠纯化DNA提取试剂盒及常规硅珠法样本图谱峰高大于DNA IQ~(TM)系统(P0.001),超高效硅珠纯化DNA提取试剂盒和常规硅珠法样本图谱峰高大于D盾超敏DNA提取试剂盒(P0.01)。结论 D盾超敏DNA提取试剂盒、超高效硅珠纯化DNA提取试剂盒及常规硅珠法对于滤纸血痕的DNA提取效率高于DNA IQ~(TM)系统;超高效硅珠纯化DNA提取试剂盒和常规硅珠提取到的DNA溶液可能具有更高的质量。     

Maxwell 16裂解纯化法提取陈旧精子DNA的应用

目的利用Maxwell 16裂解纯化法从保存8年以上陈旧精斑检材中获取精子DNA。方法 8份陈旧精斑检材采用Maxwell 16裂解纯化法提取精子DNA,并采用Powerplex○R21试剂盒进行复合扩增,产物用AB3130型遗传分析仪检测,结果与常规方法进行对比。结果成功获得8份陈旧精斑检材精子STR分型。结论差异裂解配合Maxwell 16裂解在陈旧精斑检材精子DNA检验中效果明显。     

改良硅珠法提取DNA的灵敏性及稳定性评价初探

目的通过比较对改良硅珠法提取DNA的灵敏性和稳定性进行评价。方法样本模板使用9947A(0.1ng/μL),以30pg为等差,配置10~700pg共24种不同浓度的DNA模板,分别采用常规硅珠法与改良硅珠法提取并纯化模板DNA,在Gene Amp PCR System 9700上进行PCR扩增,ABI 3500XL型荧光分析仪进行电泳检测。结果与9947A标准品阳性对照比较,采用常规硅珠法检验,24份样本均未获得成功分型;采用改良硅珠法检验,当模板量达到550pg时,即可得到所有基因座的成功分型;模板量达到580pg及以上时,16个基因座图谱峰值均可超过200RFU,分型稳定准确。结论改良硅珠法提取DNA易于操作,稳定性较好,灵敏度优于常规硅珠法,可在法医微量物证DNA检验中应用。     

wizard clean up在混合斑DNA检验中的应用

目的建立一种快速、简单、有效的混合斑DNA检验方法。方法在100例检案中,利用wizardcleanup直接对精子消化液进行纯化浓缩。采用profilerplus试剂盒进行复合扩增,产物经ABI310基因分析仪检测。结果从混合斑中成功获得精斑10个STR位点的DNA分型。结论wizardcleanup处理混合斑,能有效去除女性成份,得到精斑DNA进行分型。     

3种提取胶带粘面汗潜指印中DNA的方法比较

目的比较胶带粘面汗潜指印中DNA提取的方法。方法分别采用硅珠法、QIAMicrokit法、硅珠-QIAMicrokit法提取胶带粘面的汗潜指印中DNA,STR复合扩增,荧光电泳检测。结果用QIAMicrokit法、硅珠-QIAMicrokit法提取胶带粘面汗潜指印中DNA,检测成功率分别为21%和36%。硅珠法检测未获成功。结论硅珠-QIAMicrokit法提取胶带粘面汗潜指印中的DNA比QIAMicrokit法,检验时间更短,检测成功率更高。     

磁珠法自动化纯化现场检材DNA方法研究

目的利用TE-MAGS在TECAN工作站上结合磁珠试剂盒,建立自动化工作站批量纯化现场检材DNA的方法,并探讨其在法医物证检案中的应用。方法灵敏度测试:标准品使用0.1ng/μL 9947A,用200μL TES稀释制备DNA总量0.1ng~1ng共10种的标准样品,采用本文方法提取纯化,使用IdentifilerTM试剂盒扩增,用3130XL型测序仪检测,Gene Mapper ID-X分析,分析STR图谱质量;纯化能力测试:在1ng总量的标准样品中加入腐殖酸、血红素,采用本文方法提取纯化、扩增检测,分析STR图谱质量;实际案件应用对比:收集304份现场检材,分别采用本方法和硅珠法进行提取纯化,经扩增检测,统计对比两种提取纯化方法 STR分型成功率。结果灵敏度测试:0.1ng~0.2ng总量标准样品提取的DNA模板,扩增后可检测到部分基因座STR图谱,0.3ng~1ng总量标准样品提取的DNA模板,扩增后可以得到完整的STR图谱;纯化能力测试:对混合有一定浓度的腐殖酸、血红素的标准样品的提取产物检测图谱未见明显抑制;实际案件应用对比测试:304份现场检材工作站磁珠法检出成功率(50%)高于硅珠法(40.8%)。结论本文所建立的方法缓冲范围较大,回收率高,纯化能力强,提取产物STR分型成功率高,适合现场检材批量化DNA检验。     

wiazrd clean up在混合斑DNA检验中的应用

目的 建立一种快速、简单、有效的混合斑DNA检验方法。方法 在100例检案中，利用wizard clean up直接对于精子消化液进行纯化浓缩。采用profiler plus试剂盒进行复合扩增，产物经ABI310基因分析仪检测。结果 从混合斑中成功获得精斑10个STR位点的DNA分型。结论 wizard clean up处理混合斑，能有效去除女性成份，得到精斑DNA进行分型。     

改良EVO150-8方法在DNA自动化检案中的应用

目的探讨改良EVO150-8方法在批量生物检材DNA检验中的应用价值,建立一种自动化、简单、快速的DNA提取方法。方法采用改良EVO150-8自动化核酸提取纯化仪器与DNA IQ磁珠法纯化试剂盒,对各现场提取的880份血迹、烟蒂、口香糖、精斑（混合斑）、组织、骨骼、脱落细胞等常见生物检材进行DNA提取与纯化,采用Identifiler试剂盒进行扩增检验,用3130XL电泳,GeneMapper ID V3.2分析软件进行分析比对。结果在880份生物检材中,有836份检材成功获得STR分型;检验92份检材仅需时128min。结论改良EVO150-8适合批量生物检材的自动化提取。     

P30试验阴性检出精子基因型1例

1案例某男怀疑其女友有外遇,自行提取女友黑色三角内裤一件送检,要求检验是否含人精斑。接案后,按照精斑检验常规,进行酸性磷酸酶(磷酸苯二钠)预试验和胶体金P30抗原检测试剂条(购自公安部物证鉴定中心)试验,结果均呈阴性,阴阳性对照结果准确。沉渣涂片,HE染色,镜下见有大量精子,透明顶体明显,大小一致,未能见明显尾部;分步消化后用硅珠法提取DNA,经荧光标记STR复合扩增技术,检出样品中15个位点的男性DNA。2讨论酸性磷酸酶(磷酸苯二钠)试验灵敏度较高,稀释20000倍的精液仍呈阳性反应;P30为前列腺特异性抗原(prostatespecificantigen P…     

Development of a one-tube extraction and amplification method for DNA analysis of sperm and epithelial cells recovered from forensic samples by laser microdissection

Laser microdissection can be used in forensic casework to isolate specific cell types from mixtures of biological samples. Extraction of DNA from selected cells is still required prior to STR amplification. Because of the relatively pristine nature of the recovered cells, laser microdissection is more sensitive than more traditional methods of DNA analysis, theoretically resulting in DNA profiles from less cellular material. A one-tube extraction and amplification method minimises loss of DNA through liquid transfers and reduces the potential for contamination events occurring. In this paper, the development of a one-tube method for the effective extraction of DNA from laser microdissected sperm and epithelial cells is described. The performance of the in-house method was compared to that of a commercial DNA extraction kit for extraction of DNA from sperm and the downstream compatibility with STR amplification was determined for both sperm and epithelial samples. Full Identifiler™ profiles after 28 amplification cycles were obtained from as few as 15 epithelial cells and 30 sperm.     

HE染色涂片上精子DNA的提取与HLA-DQa基因扩增分型

本文对ＨＥ染色涂片上精子ＤＮＡ的提取、ＰＣＲ扩增分型的可行性与可靠性进行了研究。２０张ＨＥ染色涂片的实验结果表明：ＨＥ染色涂片上的精子是可以被回收并提取到ＤＮＡ进行ＨＬＡ－ＤＱａ基因的ＰＣＲ扩增分型的，其分型结果准确可靠。这说明精子的ＨＥ染色涂片也是进行ＤＮＡ分析的一种很好的检材来源。     

The modified method of two-step differential extraction of sperm and vaginal epithelial cell DNA from vaginal fluid mixed with semen

This investigation was undertaken as an efficient method for isolating sperm DNA from a mixed fluid sample which contains vaginal epithelial cells in a greater amount. The modified method of the two-step differential extraction procedure was found to be suitable for separating sperm DNA and vaginal epithelial cell DNA from the mixed stains. As the first step of digestion, vaginal epithelial cells in the mixed stains were lysed with Proteinase K and SDS, and sperm heads remaining in the lysed solution were collected by centrifugation. As the second step digestion, the sperm heads were lysed with the buffer containing Proteinase K, SDS and DTT as reducing agent. DNA fractions extracted from the two lysed solutions were enriched, one with sperm DNA and the other with vaginal epithelial cell DNA. MCT118(D1S80), ApoB VNTR and HLADQα types of sperm DNA were detected and were confirmed by matching with corresponding male blood DNA. In the case of vaginal secretion mixed with semen of two males, the mixture of MCT118 types of the two males was detected in sperm DNA fraction.     

改良差异裂解法结合硅珠法提取混合斑精子DNA

目的采用改良差异裂解法结合硅珠法提取混合斑中精子DNA,并评价其应用价值。方法收集52例经常规差异裂解法检验含有女性分型的混合斑检材,采用改良差异裂解法结合硅珠法提取精子细胞DNA,IdentifilerTM试剂盒进行PCR扩增检验。并将常规差异裂解法结果作为对照。结果52例混合斑检材中,采用改良差异裂解法结合硅珠法检出单一男性精子成分有38例,男性分型检出率达到98．08％。结论改良差异裂解法结合硅珠法适合提取混合斑中精子DNA。     

3种DNA提取法在污染严重混合斑分型中的应用比较

目的比较Chelex-100法、酚/氯仿法和二氧化硅膜法3种DNA提取法在污染严重混合斑分型中的应用效果。方法从日常案例中收集污染严重的混合斑25份,差异消化法分离精子后同时用Chelex-100法、酚/氯仿法和二氧化硅膜技术3种方法提取DNA,采用PCR-STR技术对D19S253、FGA和CSF1PO 3个基因座进行分型,Gel-Pro软件处理电泳图谱,SPSS软件分析比较不同方法之间的差异。结果采用Chelex-100法提取DNA,25份检材分型结果均未成功;采用酚/氯仿法,25份检材中10份分型成功,3份检材FGA和CSF1PO基因座可分型,4份检材CSF1PO基因座可分型;采二氧化硅膜纯化法,25份检材均成功分型;酚/氯仿法和二氧化硅膜法两种方法比较,结果存在显著性差异(P<0.05)。结论二氧化硅膜纯化技术可以有效去除PCR抑制物,提取的DNA扩增效果明显优于Chelex-100法和酚/氯仿法,具有较高的应用价值。     

不同保存时间和不同精子数量精斑样本DNA分型比较

目的比较不同保存时间和不同精子数量精斑样本DNA分型的效果。方法制备精斑样本,保存10d的样本采用激光显微捕获30、20、15、10、5、1个精子,用于不同数量精子分型比较;保存10d、214d、375d的样本分别捕获30、20、10个精子,用于不同保存时间分型比较。比较各组检出率、等位基因丢失率和非特异性扩增率,采用χ2检验进行差异比较。结果①不同精子数量分型：捕获10个精子即可得到完整的DNA分型,且随着精子数增多,检出率逐渐提高而等位基因丢失率逐渐降低,30个精子等位基因丢失率为0%,1个精子则可达58.89%;②不同保存时间分型：总趋势是保存时间越短,捕获精子越多检出率越高,10个精子与20、30个精子组比较,均有显著性差异（P〈0.05）;等位基因丢失率及非特异性扩增率则随保存时间的延长而增加,相同保存时间的不同精子数量组之间和相同的精子数量的不同保存时间组之间比较,差异均具有统计学意义（P〈0.05）。结论激光显微捕获精子数目和检材保存时间对DNA分型结果有直接影响。     

精子细胞定向捕获与分离技术初步研究

目的探索并研究精子细胞定向捕获与分离技术,初步建立精子细胞特异性分离与DNA提取的方法与试剂体系。方法通过特异性定向捕获复合体（精子特异性抗体一磁性纳米微球）的制备,在一定的试剂体系环境下,实现精子细胞的定向捕获与分离。结果能够实现精子细胞的定向富集与分离,通过后续的提取过程,获得了高质量的DNA,并获得了相应的完整STR分型结果。     

Microchip-based cell lysis and DNA extraction from sperm cells for application to forensic analysis

The current backlog of casework is among the most significant challenges facing crime laboratories at this time. While the development of next-generation microchip-based technology for expedited forensic casework analysis offers one solution to this problem, this will require the adaptation of manual, large-volume, benchtop chemistry to small volume microfluidic devices. Analysis of evidentiary materials from rape kits where semen or sperm cells are commonly found represents a unique set of challenges for on-chip cell lysis and DNA extraction that must be addressed for successful application. The work presented here details the development of a microdevice capable of DNA extraction directly from sperm cells for application to the analysis of sexual assault evidence. A variety of chemical lysing agents are assessed for inclusion in the extraction protocol and a method for DNA purification from sperm cells is described. Suitability of the extracted DNA for short tandem repeat (STR) analysis is assessed and genetic profiles shown. Finally, on-chip cell lysis methods are evaluated, with results from fluorescence visualization of cell rupture and DNA extraction from an integrated cell lysis and purification with subsequent STR amplification presented. A method for on-chip cell lysis and DNA purification is described, with considerations toward inclusion in an integrated microdevice capable of both differential cell sorting and DNA extraction. The results of this work demonstrate the feasibility of incorporating microchip-based cell lysis and DNA extraction into forensic casework analysis.     

Expedited, chemically enhanced sperm cell recovery from cotton swabs for rape kit analysis

This report focuses on the development of a method for chemically induced enhancement of cell elution and recovery from cotton swabs. The method exploits the exclusive use of detergents for intact cell removal, and can be utilized in conjunction with, or to circumvent, conventional differential extraction (DE). Samples treated with Sarkosyl (54.4 +/- 1.8%) and sodium dodecyl sulfate (SDS) (78.5 +/- 0.7%) yielded higher sperm cell recoveries than a conventional DE buffer (39.4 +/- 2.1%). The results indicated that the choice of detergent affected sperm cell yield, with anionic detergents having the greatest effect. Storage time of samples affected the concentration of detergent required for optimal sperm cell recovery, longer times requiring increased detergent concentrations. In addition, the extent of sperm cell lysis by proteinase K digestion was evaluated. The results indicate that the exclusive use of SDS enhances the release of sperm and epithelial cells from a cotton swab as compared with DE buffer, providing for a more effective DNA analysis.