Evaluation of Non-Formalin Tissue Fixation for Molecular Profiling Studies

Gillespie, John W.; Best, Carolyn J.M.; Bichsel, Verena E.; Cole, Kristina A.; Greenhut, Susan F.; Hewitt, Stephen M.; Ahram, Mamoun; Gathright, Yvonne; Merino, María J.; Strausberg, Robert L.; Epstein, Jonathan I.; Hamilton, Stanley R.; Gannot, Gallya; Baibakova, Galina V.; Calvert, Valerie; Flaig, Michael J.; Chuaqui, Rodrigo F.; Herring, Judi; Pfeifer, John D.; Petricoin, Emanuel F.; Linehan, W. Marston; Duray, Paul H.; Bova, G. Steven; Emmert‐Buck, Michael R.

doi:10.1016/s0002-9440(10)64864-x

Cited by 264 publications

(209 citation statements)

References 29 publications

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“…In a previous study on the effect of fixatives on the preservation, we also assessed the use of alternative embedding procedures, such as low-temperature melting polyester wax. 1 Higher and more intense RNA smears were seen when embedding was performed with low-temperature melting polyester waxes ( Figure 6A from reference 1 ). This data suggests that in addition to fixation, the conventional paraffin-embedding step, used in most of the laboratories, also significantly influences RNA stability.…”

Section: Discussionmentioning

confidence: 96%

“…We have recently demonstrated the utility of an alternative fixation method, 70% ethanol followed by paraffin embedding. 1 The advantages of formalin-fixed samples are maintained, including excellent preservation of visual details, while allowing for the recovery and analysis of biomolecules. [1][2][3] For example, RT-PCR for specific genes can be performed on RNA from ethanol-paraffin tissues, including small samples such as microdissected cells.…”

Section: (J Mol Diagn 2004 6:371-377)mentioning

confidence: 99%

“…[1][2][3] For example, RT-PCR for specific genes can be performed on RNA from ethanol-paraffin tissues, including small samples such as microdissected cells. 1 However, an in-depth evaluation of the global integrity of mRNA in ethanol-paraffin samples has not been performed.…”

Section: (J Mol Diagn 2004 6:371-377)mentioning

confidence: 99%

“…Ethanol fixation and paraffin embedding followed previously established protocols. 1 Specimens obtained from patients on an IRBapproved protocol at the Catholic University in Santiago, Chile, were snap-frozen in OCT and stored at Ϫ80°C. Three frozen cases (Fr1, Fr2, and Fr3) and three ethanolfixed, paraffin-embedded cases (EP1, EP2, and EP3) were selected for microdissection to obtain matched benign prostatic hyperplasia (BPH) and prostate carcinoma cells.…”

Section: Tissue Preservation and Laser Capture Microdissectionmentioning

confidence: 99%

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Comparison of Snap Freezing versus Ethanol Fixation for Gene Expression Profiling of Tissue Specimens

Perlmutter

Best

Gillespie

et al. 2004

The Journal of Molecular Diagnostics

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Frozen tissue specimens are the gold standard for molecular analysis. However, snap freezing presents several challenges regarding collection and storage of tissue, and preservation of histological detail. We evaluate an alternative preservation method, ethanol fixation followed by paraffin embedding, by analyzing expression profiles of microdissected cells on Affymetrix oligonucleotide arrays of three matched benign prostatic hyperplasia (BPH) and tumor samples processed with each preservation method. Frozen samples generated an average present call of 26% of the probe sets, compared to 4.5% in ethanol-paraffin samples. Eighty-eight percent of the probe sets called present in the ethanol-paraffin samples were also present in the frozen specimens. Comparing ethanolparaffin BPH to tumor, 52 probe sets showed a twofold differential expression or higher in at least two cases, 23 of which were also differentially expressed in at least one frozen case. Despite a significant drop in the number of transcripts detectable, the data suggests that the obtainable information in ethanol-fixed samples may be useful for molecular profiling where frozen tissue is not available. However, ethanol fixation and paraffin embedding of tissue specimens is not optimal for high-throughput mRNA expression analysis. Improved methods for transcript profiling of archival samples, and/or tissue processing are still required. Formalin fixation and paraffin embedding is the standard tissue processing method used in histopathology laboratories. This protocol allows for permanent preservation of the tissues, easy storage, and optimal histological quality. Unfortunately, formalin fixation severely compromises analysis of biomolecules, in particular mRNA and proteins. We have recently demonstrated the utility of an alternative fixation method, 70% ethanol followed by paraffin embedding. 1

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Section: Discussionmentioning

confidence: 96%

Section: (J Mol Diagn 2004 6:371-377)mentioning

confidence: 99%

Section: (J Mol Diagn 2004 6:371-377)mentioning

confidence: 99%

Section: Tissue Preservation and Laser Capture Microdissectionmentioning

confidence: 99%

See 2 more Smart Citations

Comparison of Snap Freezing versus Ethanol Fixation for Gene Expression Profiling of Tissue Specimens

Perlmutter

Best

Gillespie

et al. 2004

The Journal of Molecular Diagnostics

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“…First, fixation should not affect RNA integrity/quality as a prerequisite for downstream analysis by RNA-seq and second, it should not interfere with GFP fluorescence as this parameter is the basis for FACS-based discrimination of host populations. Here, seven commonly used fixation methods were tested with regard to these two parameters ( Fig (Gillespie et al, 2002), the addition of 'stop solution' (i.e. 95% EtOH/5% phenol) (Eriksson et al, 2003), using the (NH4)2SO4-based reagent RNAlater (Qiagen), or different concentrations of paraformaldehyde (PFA) with or without 2% sucrose (W.-D. Hardt, personal communication).…”

Section: Transcriptome Fixationmentioning

confidence: 99%

Dual RNA-seq of pathogen and host

2012

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SummaryThe infection of a eukaryotic host cell by a bacterial pathogen is one of the most intimate examples of cross-kingdom interactions in biology. Infection processes are highly relevant from both a basic research as well as a clinical point of view. Sophisticated mechanisms have evolved in the pathogen to manipulate the host response and vice versa host cells have developed a wide range of anti-microbial defense strategies to combat bacterial invasion and clear infections.However, it is this diversity and complexity that makes infection research so challenging to technically address as common approaches have either been optimized for bacterial or eukaryotic organisms. Instead, methods are required that are able to deal with the often dramatic discrepancy between host and pathogen with respect to various cellular properties and processes. One class of cellular macromolecules that exemplify this host-pathogen heterogeneity is given by their transcriptomes: Bacterial transcripts differ from their eukaryotic counterparts in many aspects that involve both quantitative and qualitative traits. The entity of RNA transcripts present in a cell is of paramount interest as it reflects the cell's physiological state under the given condition. Genome-wide transcriptomic techniques such as RNA-seq have therefore been used for single-organism analyses for several years, but their applicability has been limited for infection studies.The present work describes the establishment of a novel transcriptomic approach for infection biology which we have termed "Dual RNA-seq". Using this technology, it was intended to shed light particularly on the contribution of non-protein-encoding transcripts to virulence, as these classes have mostly evaded previous infection studies due to the lack of suitable methods. The performance of Dual RNA-seq was evaluated in an in vitro infection model based on the important facultative intracellular pathogen Salmonella enterica serovar Typhimurium and different human cell lines. Dual RNA-seq was found to be capable of capturing all major bacterial and human transcript classes and proved reproducible. During the course of these experiments, a previously largely uncharacterized bacterial small non-coding RNA (sRNA), referred to as STnc440, was identified as one of the most strongly induced genes in intracellular Salmonella.Interestingly, while inhibition of STnc440 expression has been previously shown to cause a virulence defect in different animal models of Salmonellosis, the underlying molecular mechanisms have remained obscure. Here, classical genetics, transcriptomics and biochemical assays proposed a complex model of Salmonella gene expression control that is orchestrated by this sRNA. In particular, STnc440 was found to be involved in the regulation of multiple bacterial target mRNAs by direct base pair interaction with consequences for Salmonella virulence and

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Laser Microdissection

Frost

Eltoum

Siegal

et al. 2015

CP Molecular Biology

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Laser microdissection (LM) offers a relatively rapid and precise method of isolating and removing specified cells from complex tissues for subsequent analysis of their RNA, DNA, protein or metabolite content, thereby allowing assessment of the role of different cell types in the normal physiological or disease processes being studied. In this unit, protocols for the preparation of mammalian frozen tissues, fixed tissues, and cytologic specimens for LM, including tissue freezing, tissue processing and paraffin embedding, histologic sectioning, cell processing, hematoxylin and eosin staining, immunohistochemistry, and image-guided cell targeting are presented. Also provided are recipes for generating lysis buffers for the recovery of nucleic acids and proteins. The Commentary section addresses the types of specimens that can be utilized for LM and approaches to staining of specimens for cell visualization. Emphasis is placed on the preparation of tissue or cytologic specimens as this is critical to effective LM.

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Evaluation of Non-Formalin Tissue Fixation for Molecular Profiling Studies

Cited by 264 publications

References 29 publications

Comparison of Snap Freezing versus Ethanol Fixation for Gene Expression Profiling of Tissue Specimens

Comparison of Snap Freezing versus Ethanol Fixation for Gene Expression Profiling of Tissue Specimens

Dual RNA-seq of pathogen and host

Laser Microdissection

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