Identification of apolipoprotein E polymorphisms using temperature cycled primer oligo base extension and mass spectrometry.

D P Little, A Braun, B Darnhofer-Demar, H Köster
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引用次数: 0

Abstract

The isothermal Primer Oligo Base Extension (PROBE) reaction combined with matrix-assisted laser desorption/ionization time-of-flight mass spectrometry for diagnostic product detection as recently introduced by our group is modified to incorporate temperature cycling during the primer extension step, resulting in enhanced levels of diagnostic product generation. Utilizing temperature cycled PROBE, the identities of two apolipoprotein E polymorphisms (codons 112 and 158) for differentiation of epsilon 2/epsilon 3, epsilon 3/epsilon 3, epsilon 3/epsilon 4, and epsilon 4/epsilon 4 genotypes were simultaneously determined. Primers specific for each site are extended by a series of bases unique to the identity of that variable site, producing low mass diagnostic products (M(r) < 9000) highly amenable to detection by mass spectrometry. The temperature cycled PROBE method has yielded unambiguous and correct diagnoses for all samples tested thus far. The increased amount of diagnostic product generated per primer by the cycling method makes possible faster spectrum acquisition due to the increased signal intensity, critical for future automated measurement of such samples.

利用温度循环引物寡核苷酸延伸和质谱法鉴定载脂蛋白E多态性。
我们小组最近推出的用于诊断产品检测的等温引物Oligo碱基延伸(PROBE)反应结合基质辅助激光解吸/电离飞行时间质谱法,在引物延伸步骤中加入温度循环,从而提高了诊断产品的生成水平。利用温度循环探针,同时确定了两种载脂蛋白E多态性(密码子112和158)对epsilon 2/epsilon 3、epsilon 3/epsilon 3、epsilon 3/epsilon 4和epsilon 4基因型分化的身份。针对每个位点的特异引物由一系列针对该可变位点的独特碱基延伸,产生低质量诊断产品(M(r) < 9000),高度适合于质谱检测。到目前为止,温度循环探针方法对所有测试的样品都产生了明确和正确的诊断。由于信号强度的增加,循环方法每个引物产生的诊断产品数量的增加使得更快的频谱采集成为可能,这对未来此类样品的自动化测量至关重要。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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