Total RNA extraction from tissues for microRNA and target gene expression analysis: not all kits are created equal

Brown, Rikki A. M.; Epis, Michael R.; Horsham, Jessica L.; Kabir, Tasnuva D.; Richardson, Kirsty; Leedman, Peter J.

doi:10.1186/s12896-018-0421-6

Cited by 95 publications

(57 citation statements)

References 32 publications

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“…However, it is still difficult to quantify the levels of c-miRNAs due to their low concentrations while all the miRNA detection methods depend on the quality of the starting material. In addition, the most widely used methods including qRT-PCR and microarray are based on the assumption that the different RNA extraction methods isolate all miRNAs equally [29]. However, as discussed above the levels of c-miRNA isolated using different methods should not be directly compared as the recovery of c-miRNA varies dramatically [127,128].…”

Section: Detection Methods and Normalization Strategiesmentioning

confidence: 99%

“…Additionally, due to their low concentration in plasma and serum, miRNAs can only be quantified using amplification techniques and thus the amount of starting material and the extraction method may affect the results [28]. It has been demonstrated that sample type and processing, as well as RNA extraction methods significantly affect the miRNA profile and/or expression levels [28,29]. Importantly, a comparison of c-miRNA profiles obtained by different laboratories for the same disease, including CVDs, revealed different expression levels of specific miRNAs (see [30] and references cited therein), illustrating the need to standardize the detection and analysis of c-miRNAs.…”

Section: Introductionmentioning

confidence: 99%

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Challenges in Using Circulating Micro-RNAs as Biomarkers for Cardiovascular Diseases

Felekkis

Papaneophytou

2020

IJMS

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Micro-RNAs (miRNAs) play a pivotal role in the development and physiology of the cardiovascular system while they have been associated with multiple cardiovascular diseases (CVDs). Several cardiac miRNAs are detectable in circulation (circulating miRNAs; c-miRNAs) and are emerging as diagnostic and therapeutic biomarkers for CVDs. c-miRNAs exhibit numerous essential characteristics of biomarkers while they are extremely stable in circulation, their expression is tissue-/disease-specific, and they can be easily detected using sequence-specific amplification methods. These features of c-miRNAs are helpful in the development of non-invasive assays to monitor the progress of CVDs. Despite significant progress in the detection of c-miRNAs in serum and plasma, there are many contradictory publications on the alterations of cardiac c-miRNAs concentration in circulation. The aim of this review is to examine the pre-analytical and analytical factors affecting the quantification of c-miRNAs and provide general guidelines to increase the accuracy of the diagnostic tests in order to improve future research on cardiac c-miRNAs.

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Section: Detection Methods and Normalization Strategiesmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Challenges in Using Circulating Micro-RNAs as Biomarkers for Cardiovascular Diseases

Felekkis

Papaneophytou

2020

IJMS

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“…Then, total RNA was extracted using the phenol chloroform method (21). The purity of RNA was determined by A260/A280 using ultraviolet spectrophotometry (Nanodrop 2000 Spectrophotometer; Thermo Fisher Scientific, Inc.).…”

Section: Methodsmentioning

confidence: 99%

MicroRNA‑138 inhibits SOX12 expression and the proliferation, invasion and migration of ovarian cancer cells

Zhu

Jin

2018

Exp Ther Med

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The aim of the present study was to investigate the expression and biological functions of microRNA (miR)-138 in ovarian cancer at the tissue and cellular levels, as well as its underlying mechanisms. A total of 47 patients with ovarian cancer were included in the present study. Ovarian cancer tissues were subjected to staging classification according to the FIGO 2000 criteria. Lymphatic metastasis was also examined. Ovarian cancer A2780 cells were transfected using liposomes. Reverse transcription-quantitative polymerase chain reaction was used to measure the expression of miR-138. A Cell-Counting Kit 8 assay was used to examine cell viability, while a Transwell assay was employed to study cell invasion and migration. The effects of miR-138 on SOX12 protein expression were examined by western blot analysis. A dual luciferase reporter assay was performed to identify the direct interaction between miR-138 and SOX12 gene. Expression of miR-138 was downregulated in ovarian cancer tissues. The level of miR-138 in patients with ovarian cancer with lymphatic metastasis was significantly lower compared with patients without lymphatic metastasis. However, expression of miR-138 was not associated with the stage of ovarian cancer. Upregulation of miR-138 inhibited the proliferation and suppressed the invasion and migration of A2780 cells. SOX12 promoted the proliferation, invasion and migration of A2780 cells. In addition, miR-138 downregulated the expression of SOX12 via binding with the 3′-UTR of SOX12 gene. The present study demonstrates that miR-138 expression is downregulated in ovarian cancer tissues and miR-138 acts as a tumor suppressor gene by inhibiting SOX12 expression and the proliferation, invasion and migration of ovarian cancer cells.

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“…However no correlations between fold changes in sequencing reads and qPCR abundance for expression of miR‐100‐5p, ‐23b‐5p, and ‐203a were detected. This observed discordance again reflects the uncertainties imposed by different RNA isolation methods, in this study to undertake qPCR analysis, ‐phenol chloroform‐based extraction method was used, differing from the solid‐phase separation with affinity resin based extraction that is necessary for purifying better quality RNA needed for HTS . Further, quantification of miRNA expression by qPCR is influenced by the choice of reference genes used for normalization .…”

Section: Discussionmentioning

confidence: 99%

Comprehensive Profiling of the Circulatory miRNAome Response to a High Protein Diet in Elderly Men: A Potential Role in Inflammatory Response Modulation

Ramzan

Mitchell

Milan

et al. 2019

Molecular Nutrition Food Res

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Scope MicroRNA are critical to the coordinated post‐transcriptional regulation of gene expression, yet few studies have addressed the influence of habitual diet on microRNA expression. High protein diets impact cardiometabolic health and body composition in the elderly suggesting the possibility of a complex systems response. Therefore, high‐throughput small RNA sequencing technology is applied in response to doubling the protein recommended dietary allowance (RDA) over 10 weeks in older men to examine alterations in circulating miRNAome. Methods and Results Older men (n = 31; 74.1 ± 0.6 y) are randomized to consume either RDA (0.8 g kg−1 day−1) or 2RDA (1.6 g kg−1 day−1) of protein for 10 weeks. Downregulation of five microRNAs (miR‐125b‐5p, ‐100‐5p, ‐99a‐5p, ‐23b‐3p, and ‐203a) is observed following 2RDA with no changes in the RDA. In silico functional analysis highlights target gene enrichment in inflammation‐related pathways. qPCR quantification of predicted inflammatory genes (TNFα, IL‐8, IL‐6, pTEN, PPP1CB, and HOXA1) in peripheral blood mononuclear cells shows increased expression following 2RDA diet (p ≤ 0.05). Conclusion The study findings suggest a possible selective alteration in the post‐transcriptional regulation of the immune system following a high protein diet. However, very few microRNAs are altered despite a large change in the dietary protein.

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Total RNA extraction from tissues for microRNA and target gene expression analysis: not all kits are created equal

Cited by 95 publications

References 32 publications

Challenges in Using Circulating Micro-RNAs as Biomarkers for Cardiovascular Diseases

Challenges in Using Circulating Micro-RNAs as Biomarkers for Cardiovascular Diseases

MicroRNA‑138 inhibits SOX12 expression and the proliferation, invasion and migration of ovarian cancer cells

Comprehensive Profiling of the Circulatory miRNAome Response to a High Protein Diet in Elderly Men: A Potential Role in Inflammatory Response Modulation

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