Evaluation of Quality-Control Criteria for Microarray Gene Expression Analysis

Dumur, Catherine I.; Nasim, Suhail; Best, Al M.; Archer, Kellie J.; Ladd, Amy C.; Mas, Valeria R.; Wilkinson, David S.; Garrett, Carleton T.; Ferreira‐Gonzalez, Andrea

doi:10.1373/clinchem.2004.033225

Cited by 99 publications

(96 citation statements)

References 18 publications

(12 reference statements)

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“…Quality control criteria included cDNA and cRNA synthesis products within median lengths of 2.0 and 3.0 kb, respectively, and 3ʹ/5ʹ ratios close to 1.00 for the housekeeping genes, GAPDH and β-actin. 8 The "significance-score" algorithm (S-score) developed by Dr. Li Zhang was used to produce a score for the comparisons of the expression summaries between cell groups. 48 The Minimum Information About a Microarray Experiment guidelines have been met, and the microarray raw data have been deposited with the National Center for Biotechnology Institute Gene Expression Omnibus-accession number GSE22578.…”

Section: Gene Expression Profilingmentioning

confidence: 99%

Novel report of expression and function of CD97 in malignant gliomas: correlation with Wilms tumor 1 expression and glioma cell invasiveness

Chidambaram

Fillmore

Meter

et al. 2012

JNS

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Object. The Wilms tumor 1 (WT1) protein-a developmentally regulated transcription factor-is aberrantly expressed in gliomas and promotes their malignant phenotype. However, little is known about the molecular allies that help it mediate its oncogenic functions in glioma cells.Methods. The authors used short interfering RNA (siRNA) to suppress WT1 expression in glioblastoma (GBM) cells and evaluated the effect of this on GBM cell invasiveness. Gene expression analysis was then used to identify the candidate genes that were altered as a result of WT1 silencing. One candidate target, CD97, was then selected for further investigation into its role by suppressing its expression using siRNA silencing, followed by proliferation and invasion assays.Results. WT1 levels were reliably and reproducibly suppressed by siRNA application. This resulted in a significant decrease in cellular invasiveness. Microarray analyses identified the gene products that were consistently downregulated (27) and upregulated (11) with WT1 silencing. Of these, CD97 expression was consistently suppressed across the 3 different GBM cell lines studied and was found on further investigation to significantly impact GBM cell invasiveness.Conclusions. Although CD97 expression in gliomas has not been described previously, we conclude that the possible upregulation of CD97 mediated by WT1 promotes cellular invasiveness-one of the most characteristic and challenging aspects of glial tumor cells. Further studies are needed to clarify the nature of this regulation and its impact, as CD97 could represent a novel target for antiglioma therapies. (http://thejns.org/doi/abs/10.3171/2011.11.JNS111455) Key Words • Wilms tumor 1 • glioblastoma • invasiveness • target genes • oncology 843Abbreviations used in this paper: ATP = adenosine triphosphate; EGF = epidermal growth factor; GBM = glioblastoma; PDGF = platelet-derived growth factor; qRT-PCR = quantitative reverse transcriptase polymerase chain reaction; SDS = sodium dodecyl sulfate; siRNA = short interfering RNA; VCU = Virginia Commonwealth University; WT1 = Wilms tumor 1.

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Section: Gene Expression Profilingmentioning

confidence: 99%

Novel report of expression and function of CD97 in malignant gliomas: correlation with Wilms tumor 1 expression and glioma cell invasiveness

Chidambaram

Fillmore

Meter

et al. 2012

JNS

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“…For Affymetrix analyses, the quality of input RNA and the consistency of sample collection and processing methods have been identified as crucial factors. Dumur and colleagues 7 recently described QC criteria for input sample RNA derived from a variety of sources, and similar criteria have been recommended in a recent best practices document from the Tumor Analysis Best Practices Working Group. 8 Once preanalytical variation has been reduced as much as possible, the analytical precision of the assay becomes the single biggest factor in determining what level of biological change can be seen.…”

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confidence: 99%

Precision Profiling and Components of Variability Analysis for Affymetrix Microarray Assays Run in a Clinical Context

Daly

Dumaual

Dotson

et al. 2005

The Journal of Molecular Diagnostics

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Although gene expression profiling using microarray technology is widely used in research environments, adoption of microarray testing in clinical laboratories is currently limited. In an attempt to determine how such assays would perform in a clinical laboratory, we evaluated the analytical variability of Affymetrix microarray probesets using two generations of human Affymetrix chips (U95Av2 and U133A). The study was designed to mimic potential clinical applications by using multiple operators, machines, and reagent lots, and by performing analyses throughout a period of several months. A mixed model analysis was used to evaluate the relative contributions of multiple factors to overall variability, including operator, instrument, run, cRNA/cDNA synthesis, and changes in reagent lots. Under these conditions, the average probeset coefficient of variation (CV) was relatively low for present probesets on both generations of chips (mean coefficient of variation, 21.9% and 27.2% for U95Av2 and U133A chips, respectively). The largest contribution to overall variation was chip-to-chip (residual) variability, which was responsible for between 40 to 60% of the total variability observed. Changes in individual reagent lots and instrumentation contributed very little to the overall variability. We conclude that the approach demonstrated here could be applied to clinical validation of Affymetrixbased assays and that the analytical precision of this technique is sufficient to answer many biological questions. (J Mol Diagn 2005, 7:404 -412)

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“…With this extensive preliminary conceptual profiling and practical gene array experience, we have proposed a prospective, longitudinal, multicenter study to answer these questions. We are also aware of the limitations that can arise from the rigorous criteria for total RNA quality, cDNA and cRNA synthesis, and hybridization to ensure reproducible and accurate microarray data (24) and the need for multicenter patient contribution to eliminate sample size misleading associations as occurred for patient 20 in this study.…”

Section: Discussionmentioning

confidence: 99%

“…To be considered for microarray analysis, the RNA samples needed to pass quality control criteria as 28S/18S ratios greater than 1.5 and A260nm/A280nm greater than 2.0. We established a cutoff value of 30% rRNA contribution to the total area under the electropherogram for RNA samples to be considered as intact or undegraded (24).…”

Section: Quality Controlmentioning

confidence: 99%

“…Products of cDNA synthesis and IVT were tested using the Agilent 2100 Bionalyzer (cDNA synthesis 1.5 kb < cDNA < 5.0 kb; IVT 1.0 kb < cRNA < 4.5 kb) (24). Finally, the values for a ratio of 3′/5′ for 2 housekeeping genes were checked: glyceraldehyde 3-phosphate dehydrogenase (GAPDH) and β-actin; ratios no higher than 3.00 were considered acceptable.…”

Section: Quality Controlmentioning

confidence: 99%

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Differentially Expressed Genes between Early and Advanced Hepatocellular Carcinoma (HCC) as a Potential Tool for Selecting Liver Transplant Recipients

Mas

Maluf

Archer

et al. 2006

Mol Med

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Hepatocellular carcinoma (HCC) is the fifth most common cancer in the world. Liver transplantation (LT) represents a curative treatment for "small" HCC. Preoperative staging is critical in selecting optimal candidates for LT to optimize the use of this scarce resource. From December 1997 to February 2004, 148 patients diagnosed with cirrhosis and HCC were evaluated at our center. After staging, the patients were listed for LT according to United Network for Organ Sharing (UNOS) criteria. When pretransplant liver MRIs were compared with the findings of the explanted livers, 8 of 35 patients (22.8%) were understaged. Three of the 8 patients (37.5%) had recurrence post-LT. A retrospective gene expression profiling study was done using microarray technology for tumor samples in the pretransplant hepatitis C virus (HCV)-HCC understaged patients and in a contemporaneous group of HCV-HCC patients that were accurately staged. Two sample t tests comparing the early versus advanced HCV-HCCs with respect to gene expression showed an important set of genes differentially expressed among the samples. Hierarchical clustering analysis of the gene expression profiling classified 93.8% of the total tumor samples and 85.7% of the understaged samples in concordance with the explanted pathological staging. We found a distinctive pattern of gene expression between early and advanced HCV-HCCs. These results suggest that gene expression profiling could improve the pre-LT HCC staging to more closely mimic the explant pathology. Whether gene expression profiling of HCC will be refined to the point of predicting potential metastatic biologic behavior to predict post-LT recurrence will require longitudinal prospective study of this gene array technology.

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Evaluation of Quality-Control Criteria for Microarray Gene Expression Analysis

Cited by 99 publications

References 18 publications

Novel report of expression and function of CD97 in malignant gliomas: correlation with Wilms tumor 1 expression and glioma cell invasiveness

Novel report of expression and function of CD97 in malignant gliomas: correlation with Wilms tumor 1 expression and glioma cell invasiveness

Precision Profiling and Components of Variability Analysis for Affymetrix Microarray Assays Run in a Clinical Context

Differentially Expressed Genes between Early and Advanced Hepatocellular Carcinoma (HCC) as a Potential Tool for Selecting Liver Transplant Recipients

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