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Distortion of quantitative genomic and expression hybridization by C(o)t-1 DNA: mitigation of this effect

机译:C(o)t-1 DNA定量基因组和表达杂交的扭曲:减轻这种影响

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摘要

Cross-hybridization of repetitive sequences in genomic and expression arrays is reported to be suppressed with repeat-blocking nucleic acids (C(o)t-1 DNA). Contrary to expectation, we demonstrated that C(o)t-1 also enhanced non-specific hybridization between probes and genomic targets. When added to target DNA, C(o)t-1 enhanced hybridization (2.2- to 3-fold) to genomic probes containing conserved repetitive elements. In addition to repetitive sequences, C(o)t-1 was found to be enriched for linked single copy (sc) sequences. Adventitious association between these sequences and probes distort quantitative measurements of the probes hybridized to desired genomic targets. Quantitative microarray hybridization studies using C(o)t-1 DNA are also susceptible to these effects, especially for probes that map to genomic regions containing conserved repetitive sequences. Hybridization measurements with such probes are less reproducible in the presence of C(o)t-1 than for probes derived from sc regions or regions containing divergent repeat elements, a finding with significant ramifications for genomic and expression microarray studies. We mitigated the requirement for C(o)t-1 either by hybridizing with computationally defined sc probes lacking repeats or by substituting synthetic repetitive elements complementary to sequences in genomic probes.
机译:据报道,基因组和表达阵列中重复序列的交叉杂交被重复阻断核酸(C(o)t-1 DNA)抑制。与预期相反,我们证明了C(o)t-1还增强了探针和基因组靶标之间的非特异性杂交。当添加到目标DNA时,C(o)t-1增强了与包含保守重复元件的基因组探针的杂交(2.2到3倍)。除了重复序列,还发现C(o)t-1富含链接的单拷贝(sc)序列。这些序列与探针之间的不定联系使与所需基因组靶标杂交的探针的定量测量值失真。使用C(o)t-1 DNA进行定量微阵列杂交研究也容易受到这些影响,尤其是对于那些映射到包含保守重复序列的基因组区域的探针而言。在存在C(o)t-1的情况下,用这种探针进行的杂交测量的可重复性不如从sc区域或含有不同重复元件的区域衍生的探针,这一发现对于基因组和表达微阵列研究具有重大意义。我们通过与缺乏重复的计算定义的sc探针杂交或通过替代与基因组探针序列互补的合成重复元件来减轻对C(o)t-1的需求。

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