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Expanding the map of protein-RNA interaction sites via cell fusion followed by PAR-CLIP

机译:通过细胞融合在细胞融合中膨胀蛋白质RNA相互作用位点的地图,然后是PAR-夹

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摘要

PAR-CLIP (photoactivatable ribonucleoside-enhanced crosslinking and immunoprecipitation) facilitates the identification and mapping of protein/RNA interactions. So far, it has been limited to select cell-lines as it requires efficient 4SU uptake. To increase transcriptome complexity and thus identify additional RNAprotein interaction sites we fused HEK 293 T-Rex cells (HEK293-Y) that express the RNA binding protein YBX1 with PC12 cells expressing eGFP (PC12-eGFP). The resulting hybrids enable PAR-CLIP on a neuronally expanded transcriptome (Fusion-CLIP) and serve as a proof of principle. The fusion cells express both parental marker genes YBX1 and eGFP and the expanded transcriptome contains human and rat transcripts. PAR-CLIP of fused cells versus the parental HEK293-Y identified 768 novel RNA targets of YBX1. We were able to trace the origin of the majority of the short PAR-CLIP reads as they differentially mapped to the human and rat genome. Furthermore, Fusion-CLIP expanded the CAUC RNA binding motif of YBX1 to UCUUUNNCAUC. The fusion of HEK293-Y and PC12-eGFP cells resulted in cells with a diverse genome expressing human and rat transcripts that enabled the identification of novel YBX1 substrates. The technique allows the expansion of the HEK 293 transcriptome and makes PAR-CLIP available to fusion cells of diverse origin.
机译:PAR-CLIP(可去活超核糖核糖核糖核苷增强的交联和免疫沉淀)促进蛋白质/ RNA相互作用的鉴定和映射。到目前为止,它仅限于选择细胞系,因为它需要有效的4SU吸收。增加转录组复杂性,从而鉴定额外的RnaProotin相互作用位点,我们融合了HEGER 293 T-REX细胞(HEK293-Y),其表达具有表达EGFP(PC12-EGFP)的PC12细胞的RNA结合蛋白YBX1。所得的杂交种使得在神经扩展的转录组(融合夹)上使PAR-CLIP能够作为原理的证据。融合细胞表达父母标记基因YBX1和EGFP,并且膨胀的转录组含有人和大鼠转录物。融合细胞的PAR-CLIC与父母HEK293-Y确定了768个新型RNA靶标的YBX1。我们能够追踪大多数短PAR-夹的起源,因为它们差异映射到人和鼠基因组。此外,融合夹将YBX1的CaCaRNA绑定基序扩展到ucuuunncauc。 HEK293-Y和PC12-EGFP细胞的融合导致细胞具有不同基因组的细胞,表达人和大鼠转录物,使得能够鉴定新型YBX1底物。该技术允许HEK 293转录组的扩展,并使PAR-CLIP可用于不同起源的融合细胞。

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