Isolation of full‐size mRNA from ethanol‐fixed cells after cellular immunofluorescence staining and fluorescence‐activated cell sorting (FACS)

Esser, Charlotte; Göttlinger, Christoph; Kremer, Joachim; Hundeiker, Claudia; Radbruch, Andreas

doi:10.1002/cyto.990210411

Cited by 39 publications

(29 citation statements)

References 18 publications

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“…Diez et al (16) reported isolating RNA after using short ethanol fixation and cell sorting. However, this technique can lead to a time-dependent increase in loss of macromolecules through pores in the cell membrane and to rapid nucleic acid degradation by active or insufficiently inactivated ribonucleases (17). The present data regarding cyclin B1 expression levels demonstrated that this methodology generates confirmatory results.…”

Section: Quality Control Of Isolated Rnasupporting

confidence: 56%

“…Cell fixation, required for specific identification of populations to be sorted, may result in RNA degradation (16). In fact, routinely used fixatives such as ethanol and formaldehyde do not completely inactivate RNAses (17). In the present report, we described a new approach to separate cell cycle populations by fluorescence-activated cell sorter from live cells without cell fixation, followed by isolation of full-length mRNA from sorted cells.…”

Section: Resultsmentioning

confidence: 92%

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Separation of live cells in different phases of the cell cycle for gene expression analysis

2002

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BackgroundHomogeneity of cell populations is a basic requirement for gene expression analyses of the cell cycle, such as those based on microarrays. The most common approach to obtain specific populations is the use of synchronization methods that increase the number of cells representing a certain cell cycle stage. On the one hand, conventional synchronization usually causes undesirable effects. On the other hand, cell separation methods may imply loss of RNA quality, another limiting factor for expression profiling. We describe a new strategy to specifically separate live cells in different phases of the cell cycle (G1 and G2/M) to obtain good quality RNA for gene expression analyses.MethodsThe experimental design included sorting G1 and G2/M cells with the vital fluorochrome Hoechst 33342, followed by RNA isolation from the sorted cells.ResultsSorted living G1 and G2/M cells, analyzed by immunocytochemistry and laser scanning cytometry, showed strong enrichment. The quality and specificity of the isolated RNA were demonstrated by northern blot.ConclusionsThis new approach has many potential applications, such as expression profiling of specific cell populations after eliminating the irrelevant data produced by cells in other stages of the cycle. Cytometry 49:170–175, 2002. © 2002 Wiley‐Liss, Inc.

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Section: Quality Control Of Isolated Rnasupporting

confidence: 56%

Section: Resultsmentioning

confidence: 92%

Separation of live cells in different phases of the cell cycle for gene expression analysis

2002

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“…Thus, sorting from organ material based on intracellular markers would in many cases be an attractive option. Unfortunately, the fixation and permeabilization required for intracellular staining can be associated with RNA degradation (1)(2)(3).…”

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confidence: 99%

“…Reflecting the technical difficulties, only few studies have described molecular analysis of cells flow-sorted for intracellular protein markers (1)(2)(3). Most work has been done on cell lines (1,2), with only one study describing flow sorting from dissociated biopsy specimens (3).…”

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confidence: 99%

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Flow sorting from organ material by intracellular markers

et al. 2007

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Background: Fluorescence-activated cell sorting (FACS) is an attractive technique for gene or protein expression studies in rare cell populations. For cell types where specific surface markers are not known, intracellular markers can be used. However, this approach is currently held to be difficult, as the required fixation and permeabilization may cause protein modification and RNA degradation. Methods and Results: Using the rat thyroid gland as model, rare (parafollicular) and frequent (follicular) endocrine cell types were sorted based on immunostaining for intracellular calcitonin peptide and thyroglobulin protein expression. The sorted cells were compatible with Wes-

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Quantitative method to determine mRNA levels by reverse transcriptase-polymerase chain reaction from leukocyte subsets purified by fluorescence-activated cell sorting: Application to peripheral cannabinoid receptors

et al. 1999

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Isolation of full‐size mRNA from ethanol‐fixed cells after cellular immunofluorescence staining and fluorescence‐activated cell sorting (FACS)

Cited by 39 publications

References 18 publications

Separation of live cells in different phases of the cell cycle for gene expression analysis

Separation of live cells in different phases of the cell cycle for gene expression analysis

Flow sorting from organ material by intracellular markers

Quantitative method to determine mRNA levels by reverse transcriptase-polymerase chain reaction from leukocyte subsets purified by fluorescence-activated cell sorting: Application to peripheral cannabinoid receptors

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