Validation of common reference genes stability in exosomal mRNA‐isolated from liver and breast cancer cell lines

Gorji-Bahri, Gilar; Moradtabrizi, Niloofar; Vakhshiteh, Faezeh; Hashemi, Atieh

doi:10.1002/cbin.11556

Cited by 16 publications

(13 citation statements)

References 60 publications

(71 reference statements)

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“…A clear band of PCR products on 1% agarose gel electrophoresis ( Fig 1B ), as well as not seeing primer dimers in the related melt curves, proved the specificity of the designed primers. The efficiency and specificity of these primers except hypoxanthine phosphoribosyltransferase 1 ( HPRT1) , TATA-box binding protein ( TBP ), and actin beta ( ACTB) were also studied in exosomal RNA of hepatic and breast cancer cell lines by our team recently [ 14 ]. However, here we confirmed their efficiency and specificity in cellular RNA of three hepatic and three breast cancer cell lines.…”

Section: Resultsmentioning

confidence: 99%

“…We have recently reported the expression and stability status of reference genes for exosomal content of the same hepatic cancer cell lines as this study and SKBR3 as breast cancer cell line [ 14 ]. Interestingly, the geNorm showed almost similar stability ranking for cellular and exosomal content, in which B2M and YWHAZ were ranked as two stable reference genes (M value < 1) in Huh7, HepG2, and PLC-PRF5 cell lines.…”

Section: Discussionmentioning

confidence: 99%

“…PCR efficiency (E) was also provided using LinregPCR version 2017 software. Instead of making serial dilutions and drawing standard curves which may cause errors in PCR efficiency calculation due to common pipetting errors, the LinregPCR software calculates PCR efficiency for individual reaction via calculating the slope of the regression line in an exponential phase of the amplification curve, namely Window-of-Linearity (W-o-L) area, and reports the mean PCR efficiency of samples containing same primer pairs [ 14 , 17 ]. Using the LinregPCR software, the imported raw amplification data of each RT-qPCR run, belong to each reference gene analysis was automatically corrected for baseline adjustment, and at least 3 points were incorporated for the W-o-L area of each sample.…”

Section: Methodsmentioning

confidence: 99%

“…Reference genes and corresponding primers used in this study were the same selected and designed in our previously published articles [11,[14][15][16]. Evidences considering the usage of these reference genes in hepatic and breast cancer cell lines are presented in Table 1; not exactly the cell lines investigated in this study.…”

Section: Selection Of Reference Genes Designing the Primer Pairs And Calculation Of Pcr Efficiencymentioning

confidence: 99%

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Uncovering the stability status of the reputed reference genes in breast and hepatic cancer cell lines

2021

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Accurate and reliable relative gene expression analysis via the Reverse Transcription-quantitative Real Time PCR (RT-qPCR) method strongly depends on employing several stable reference genes as normalizers. Utilization of the reference genes without analyzing their expression stability under each experimental condition causes RT-qPCR analysis error as well as false output. Similar to cancerous tissues, cancer cell lines also exhibit various gene expression profiles. It is crucial to recognize stable reference genes for well-known cancer cell lines to minimize RT-qPCR analysis error. In this study, we showed the expression level and investigated the expression stability of eight common reference genes that are ACTB, YWHAZ, HPRT1, RNA18S, TBP, GAPDH, UBC, and B2M, in two sets of cancerous cell lines. One set contains MCF7, SKBR3, and MDA-MB231 as breast cancer cell lines. Another set includes three hepatic cancer cell lines, including Huh7, HepG2, and PLC-PRF5. Three excel-based softwares comprising geNorm, BestKeeper, and NormFinder, and an online tool, namely RefFinder were used for stability analysis. Although all four algorithms did not show the same stability ranking of nominee genes, the overall results showed B2M and ACTB as the least stable reference genes for the studied breast cancer cell lines. While TBP had the lowest expression stability in the three hepatic cancer cell lines. Moreover, YWHAZ, UBC, and GAPDH showed the highest stability in breast cancer cell lines. Besides that, a panel of five nominees, including ACTB, HPRT1, UBC, YWHAZ, and B2M showed higher stability than others in hepatic cancer cell lines. We believe that our results would help researchers to find and to select the best combination of the reference genes for their own experiments involving the studied breast and hepatic cancer cell lines. To further analyze the reference genes stability for each experimental condition, we suggest researchers to consider the provided stability ranking emphasizing the unstable reference genes.

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Section: Resultsmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Selection Of Reference Genes Designing the Primer Pairs And Calculation Of Pcr Efficiencymentioning

confidence: 99%

See 2 more Smart Citations

Uncovering the stability status of the reputed reference genes in breast and hepatic cancer cell lines

2021

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“…In particular, since exosomes are presently and commonly used to identify biomarkers in cancer, the identification of a suitable reference gene for exosome detection is also required ( 47 ). Gorji-Bahri et al ( 48 ) validated reference genes in pooled cancer exosomes, and Dai et al ( 49 ) revealed that GAPDH, YWHAZ and UBC were the most stably expressed reference genes in exosomal RNA isolated from liver and breast cancer cell lines. However, reference genes in HCC tissues and blood were not evaluated by in vitro experiments and another software analysis to determine stable housekeeping genes.…”

Section: Discussionmentioning

confidence: 99%

HMBS is the most suitable reference gene for RT‑qPCR in human HCC tissues and blood samples

et al. 2021

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Reverse transcription-quantitative (RT-q) PCR is the most feasible and useful technique for identifying and evaluating cancer biomarkers; however, the method requires suitable reference genes for gene expression analysis. The aim of the present study was to identify the most suitable reference gene for the normalization of relative gene expression in human hepatocellular carcinoma (HCC) tissue and blood samples. First, 14 candidate reference genes were selected through a systematic literature search. The expression levels of these genes ( ACTB, B2M, GAPDH, GUSB, HMBS, HPRT1, PGK1, PPIA, RPLP0, RPL13A, SDHA, TBP, TFRC and YWHAZ ) were evaluated using human multistage HCC transcriptome data (dataset GSE114564), which included normal liver (n=15), chronic hepatitis (n=20), liver cirrhosis (n=10), and early (n=18) and advanced HCC (n=45). From the 14 selected genes, five genes, whose expression levels were stable in all liver disease statuses ( ACTB, GAPDH, HMBS, PPIA and RPLP0 ), were further assessed using RT-qPCR in 40 tissues (20 paired healthy tissues and 20 tissues from patients with HCC) and 40 blood samples (20 healthy controls and 20 samples from patients with HCC). BestKeeper statistical algorithms were used to identify the most stable reference genes, of which HMBS was found to be the most stable in both HCC tissues and blood samples. Therefore, the results of the present study suggest HMBS as a promising reference gene for the normalization of relative RT-qPCR techniques in HCC-related studies.

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Identification and validation of extracellular vesicle reference genes for the normalization of RT‐qPCR data

Pinheiro,

Guilbert,

Lippens

et al. 2024

J of Extracellular Vesicle

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Extracellular vesicles (EVs) contain a plethora of biomolecules, including nucleic acids, with diverse diagnostic and therapeutic application potential. Although reverse transcription‐quantitative PCR (RT‐qPCR) is the most widely applied laboratory technique to evaluate gene expression, its applicability in EV research is challenged by the lack of universal and stably present reference genes (RGs). In this study, we identify, validate and establish SNRPG, OST4, TOMM7 and NOP10 as RGs for the normalization of EV‐associated genes by RT‐qPCR. We show the stable presence of SNRPG, OST4, TOMM7 and NOP10 in multiple cell lines and their secreted EVs (n = 12) under different (patho)physiological conditions as well as in human‐derived biofluids (n = 3). Enzymatic treatments confirm the presence of SNRPG, OST4, TOMM7 and NOP10 inside EVs. In addition, the four EV‐associated RGs are stably detected in a size‐range of EV subpopulations. RefFinder analysis reveals that SNRPG, OST4, TOMM7 and NOP10 are more stable compared to RGs established specifically for cultured cells or tissues such as HMBS, YWHAZ, SDHA and GAPDH. In summary, we present four universal and stably present EV‐associated RGs to enable normalization and thus steer the implementation of RT‐qPCR for the analysis of EV‐associated RNA cargo for research or clinical applications.

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Validation of common reference genes stability in exosomal mRNA‐isolated from liver and breast cancer cell lines

Cited by 16 publications

References 60 publications

Uncovering the stability status of the reputed reference genes in breast and hepatic cancer cell lines

Uncovering the stability status of the reputed reference genes in breast and hepatic cancer cell lines

HMBS is the most suitable reference gene for RT‑qPCR in human HCC tissues and blood samples

Identification and validation of extracellular vesicle reference genes for the normalization of RT‐qPCR data

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