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Selection of suitable reference genes for normalization of quantitative RT-PCR in peripheral blood samples of bottlenose dolphins (Tursiops truncatus)

机译:选择合适的参考基因以标准化宽吻海豚外周血样品中的定量RT-PCR(Tursiops truncatus)

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摘要

Quantitative RT-PCR is often used as a research tool directed at gene transcription. Selection of optimal housekeeping genes (HKGs) as reference genes is critical to establishing sensitive and reproducible qRT-PCR-based assays. The current study was designed to identify the appropriate reference genes in blood leukocytes of bottlenose dolphins (Tursiops truncatus) for gene transcription research. Seventy-five blood samples collected from 7 bottlenose dolphins were used to analyze 15 candidate HKGs (ACTB, B2M, GAPDH, HPRT1, LDHB, PGK1, RPL4, RPL8, RPL18, RPS9, RPS18, TFRC, YWHAZ, LDHA, SDHA). HKG stability in qRT-PCR was determined using geNorm, NormFinder, BestKeeper and comparative delta Ct algorithms. Utilization of RefFinder, which combined all 4 algorithms, suggested that PGK1, HPRT1 and RPL4 were the most stable HKGs in bottlenose dolphin blood. Gene transcription perturbations in blood can serve as an indication of health status in cetaceans as it occurs prior to alterations in hematology and chemistry. This study identified HKGs that could be used in gene transcript studies, which may contribute to further mRNA relative quantification research in the peripheral blood leukocytes in captive cetaceans.
机译:定量RT-PCR通常用作针对基因转录的研究工具。选择最佳管家基因(HKG)作为参考基因对于建立基于qRT-PCR的灵敏且可重复的测定至关重要。当前的研究旨在确定宽吻海豚(Tursiops truncatus)血液白细胞中的适当参考基因,以进行基因转录研究。从7个宽吻海豚身上收集的75个血液样本用于分析15个候选HKG(ACTB,B2M,GAPDH,HPRT1,LDHB,PGK1,RPL4,RPL8,RPL18,RPS9,RPS18,TFRC,YWHAZ,LDHA,SDHA)。使用geNorm,NormFinder,BestKeeper和比较delta Ct算法确定qRT-PCR中的HKG稳定性。结合使用所有四种算法的RefFinder的使用表明,PGK1,HPRT1和RPL4是宽吻海豚血液中最稳定的HKG。血液中的基因转录扰动可以指示鲸类的健康状况,因为它发生在血液学和化学变化之前。这项研究确定了可用于基因转录研究的HKG,这可能有助于圈养鲸类的外周血白细胞中进一步的mRNA相对定量研究。

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