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昼夜变化中视蛋白表达和常见管家基因需要全面的标准化方法来进行定量实时 PCR 分析。

Diurnal variation in opsin expression and common housekeeping genes necessitates comprehensive normalization methods for quantitative real-time PCR analyses.

机构信息

Department of Biology, University of Maryland, College Park, Maryland.

出版信息

Mol Ecol Resour. 2019 Nov;19(6):1447-1460. doi: 10.1111/1755-0998.13062. Epub 2019 Aug 7.

Abstract

To determine the visual sensitivities of an organism of interest, quantitative reverse transcription-polymerase chain reaction (qRT-PCR) is often used to quantify expression of the light-sensitive opsins in the retina. While qRT-PCR is an affordable, high-throughput method for measuring expression, it comes with inherent normalization issues that affect the interpretation of results, especially as opsin expression can vary greatly based on developmental stage, light environment or diurnal cycles. We tested for diurnal cycles of opsin expression over a period of 24 hr at 1-hr increments and examined how normalization affects a data set with fluctuating expression levels using qRT-PCR and transcriptome data from the retinae of the cichlid Pelmatolapia mariae. We compared five methods of normalizing opsin expression relative to (a) the average of three stably expressed housekeeping genes (Ube2z, EF1-α and β-actin), (b) total RNA concentration, (c) GNAT2, (the cone-specific subunit of transducin), (d) total opsin expression and (e) only opsins expressed in the same cone type. Normalizing by proportion of cone type produced the least variation and would be best for removing time-of-day variation. In contrast, normalizing by housekeeping genes produced the highest daily variation in expression and demonstrated that the peak of cone opsin expression was in the late afternoon. A weighted correlation network analysis showed that the expression of different cone opsins follows a very similar daily cycle. With the knowledge of how these normalization methods affect opsin expression data, we make recommendations for designing sampling approaches and quantification methods based upon the scientific question being examined.

摘要

为了确定感兴趣的生物体的视觉敏感度,通常使用定量逆转录聚合酶链反应 (qRT-PCR) 来定量测量视网膜中光敏感视蛋白的表达。虽然 qRT-PCR 是一种经济实惠、高通量的测量表达的方法,但它存在固有的归一化问题,会影响结果的解释,尤其是在视蛋白表达因发育阶段、光照环境或昼夜节律而异的情况下。我们在 24 小时内以 1 小时的增量测试了视蛋白表达的昼夜节律,并研究了 qRT-PCR 和来自丽鱼科鱼类 Pelmatolapia mariae 视网膜的转录组数据的波动表达水平如何影响数据集。我们比较了五种相对(a)三种稳定表达的管家基因(Ube2z、EF1-α 和 β-肌动蛋白)平均值、(b)总 RNA 浓度、(c)GNAT2(转导素的锥细胞特异性亚基)、(d)总视蛋白表达和(e)仅在相同锥细胞类型中表达的视蛋白归一化视蛋白表达的方法。相对于产生的锥细胞类型的比例进行归一化会产生最小的变化,最适合消除一天中的时间变化。相比之下,通过管家基因进行归一化会导致表达的每日变化最大,并表明锥细胞视蛋白表达的峰值出现在下午晚些时候。加权相关网络分析表明,不同锥细胞视蛋白的表达遵循非常相似的日常周期。了解这些归一化方法如何影响视蛋白表达数据,我们根据正在研究的科学问题,为设计采样方法和定量方法提出建议。

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