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Development of a single probe for documentation of chimerism following bone marrow transplantation.

机译:单一探针的开发用于记录骨髓移植后的嵌合现象。

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摘要

Although numerous genetic markers are available for studying chimerism after bone marrow transplantation (BMT), there remains a need for a practical and highly informative method that is applicable in the early posttransplantation period. Using DNA restriction-fragment-length polymorphisms (RFLPs), we have evaluated the feasibility of developing a single synthetic oligonucleotide probe to study post-BMT chimerism. We have thus tested three candidate probes, termed O-3315-32, O-3315-80, and O-AY-29, that are homologous to tandemly repetitive sequences. Our results demonstrated donor-specific and recipient-specific fragments in 11 of 11 HLA-matched sibling pairs tested using probes O-3315-32 and O-3315-80. When probe O-AY-29 was used, 14 of 17 sibling pairs showed both donor and recipient markers, one had only a recipient marker, and two were identical. We showed that each of the three synthetic probes was effective in documenting donor marrow engraftment, mixed hematopoietic chimerism, the patient's pre-BMT phenotype (by using cultured skin fibroblasts obtained after BMT), and the origin of the malignant hematopoietic cells (i.e., of donor or recipient origin) in patients who developed recurrent hematologic malignancy following BMT. Compared with the use of cloned genomic probes, there are several important advantages to the use of synthetic oligonucleotide probes in studying post-BMT chimerism. Synthetic probes have absolute hybridization specificity and can be designed to suit the purposes of an individual study, since they have adjustable specificity that can be altered by changes in the length of the probe and by changes in the hybridization temperature. A single synthetic probe analogous to several highly polymorphic loci can have a polymorphism information content sufficiently high so that all but a small percentage of BMT patients could be followed easily; for example, if a probe were complementary to three highly polymorphic unlinked loci, it would discriminate approximately 98% of sibling donor/recipient pairs. This would be accomplished using only one restriction-endonuclease digestion and only one gel electrophoresis. Since other genetic markers, e.g., red blood cell antigens, immunoglobulin allotypes, and chromosome analysis, are not uniformly informative and, in some cases, cannot be used in the early posttransplantation period, the use of synthetic oligonucleotide probes for analysis of DNA RFLP is emerging as the method of choice for studies of post-BMT chimerism. This method will allow for the development of new knowledge that has not been possible with previous methods.
机译:尽管有许多遗传标记可用于研究骨髓移植(BMT)后的嵌合体,但仍需要一种实用且高度有用的方法,该方法适用于移植后早期。我们使用DNA限制性片段长度多态性(RFLP),评估了开发单个合成寡核苷酸探针以研究BMT后嵌合现象的可行性。因此,我们测试了三个候选探针,称为O-3315-32,O-3315-80和O-AY-29,它们与串联重复序列同源。我们的结果表明,使用探针O-3315-32和O-3315-80测试了11个HLA匹配兄弟对中的11个中的供体特异性和受体特异性片段。当使用探针O-AY-29时,在17对同胞对中有14个同时显示了供体和受体标记,一个仅具有一个受体标记,而两个相同。我们显示,三种合成探针均能有效记录供体骨髓移植,混合造血嵌合体,患者的BMT前表型(通过使用BMT后获得的培养皮肤成纤维细胞)以及恶性造血细胞的起源(即BMT后出现复发性血液恶性肿瘤的患者)。与使用克隆的基因组探针相比,使用合成的寡核苷酸探针研究BMT后的嵌合现象有几个重要优势。合成探针具有绝对的杂交特异性,并且可以设计为适合单个研究的目的,因为它们具有可调节的特异性,可以通过探针长度的变化和杂交温度的变化来改变特异性。类似于几个高度多态性位点的单个合成探针可以具有足够高的多态性信息含量,从而可以轻松地跟踪除少数百分数之外的所有BMT患者。例如,如果一个探针与三个高度多态性的未连接基因座互补,则它将区分大约98%的同胞供体/受体对。仅使用一种限制性内切核酸酶消化和仅一种凝胶电泳即可完成此操作。由于其他遗传标记(例如红细胞抗原,免疫球蛋白同种异型和染色体分析)的信息不统一,并且在某些情况下,不能在移植后的早期使用,因此使用合成的寡核苷酸探针进行DNA RFLP分析新兴的BMT后嵌合体研究的选择方法。这种方法将允许开发以前的方法无法实现的新知识。

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