In situ-RT and immunolaser microdissection for mRNA analysis of individual cells isolated from epilepsy-associated glioneuronal tumors

Fassunke, Jana; Majores, Michael; Ullmann, Claudia; Elger, Christian E.; Schramm, Johannes; Wiestler, Otmar D.; Becker, Albert

doi:10.1038/labinvest.3700165

Cited by 37 publications

(20 citation statements)

References 18 publications

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“…Extension of LCM from small populations of cells to individual cells has relied on PCR amplification of cell DNA (Suarez-Quian et al, 1999;Obiakor et al, 2002;Orba et al, 2003) or the perceived need to purify the very small amount of RNA, approximately 20 pg from a single captured cell for RT and PCR (Jin et al, 2001;Parlato et al, 2002;Michel et al, 2003;Kamme et al, 2004;Lu et al, 2004;Fassunke et al, 2004). Hydraulic microdissection has also been coupled with nested-PCR amplification of genomic DNA to identify sequences in single B cells (Obiakor et al, 2002).…”

Section: Introductionmentioning

confidence: 99%

Laser capture microdissection and single-cell RT-PCR without RNA purification

Keays

Owens

Ritchie

et al. 2005

Journal of Immunological Methods

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Chronic infectious diseases of the central nervous system (CNS) are characterized by intrathecal synthesis of increased amounts of immunoglobulin G (IgG) directed against the agent that causes disease. In other inflammatory CNS diseases such as multiple sclerosis and CNS sarcoid, the targets of the humoral immune response are uncertain. To identify the IgGs expressed by individual CD38+ plasma cells seen in human brain sections, we merged the techniques of laser capture microdissection (LCM) and single-cell RT-PCR. Frozen brain sections from a patient who died of subacute sclerosing panencephalitis (SSPE), were rapidly immunostained and examined by LCM to dissect individual CD38+ cells. After cell lysis, we developed two techniques for reversetranscription (RT) of unpurified total RNA in the cell lysates. The first method performed repeated and rapid freeze-thawing, followed by centrifugation of the cell lysate into tubes for subsequent RT. The second, more successful method performed RT in situ on detergent-solubilized cells directly on the cap surface; subsequent nested PCR identified heavy and light chain sequences expressed by two-thirds of individually isolated plasma cells. These techniques will streamline the identification of gene expression products in single cells from complex tissues and have the potential to identify IgGs expressed in the CNS of inflammatory diseases of unknown etiology.

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Section: Introductionmentioning

confidence: 99%

Laser capture microdissection and single-cell RT-PCR without RNA purification

Keays

Owens

Ritchie

et al. 2005

Journal of Immunological Methods

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“…However, as formalin fixation results in fragmentation of RNA, these archives are difficult to exploit using recently developed molecular tools that allow a comprehensive analysis of gene expression patterns. [1][2][3] This has increased the efforts in recent years to establish biobanks of nonfixed frozen tissue. Together with attached relevant clinical information, these biobanks can provide researchers a reliable, organised source of human tissues for RNA-based analysis.…”

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confidence: 99%

Biobanking of fresh frozen tissue: RNA is stable in nonfixed surgical specimens

Micke

Ohshima

Tahmasebpoor

et al. 2006

Laboratory Investigation

205

145

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“…This technique has been devised to isolate distinct cell populations from their natural environment in situ not only according to morphology but also to immunophenotype criteria. [21][22][23] It has been used successfully for PCR-based gene analysis of specific cell populations in brain tissue, [24][25][26] brain vessels 27 and epithelial cells, 28,29 but to our knowledge has never been employed for genome-wide discovery. A major limitation has been the necessity to procure high quality and sufficient quantity of RNA.…”

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confidence: 99%