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Featured researches published by Carsten Schlüter.


Journal of Immunological Methods | 1996

The use of reverse transcription polymerase chain reaction to analyse large numbers of mRNA species from a single cell.

Kai-Michael Toellner; Dagmar Scheel-Toellner; Ulrike Seitzer; Raimund Sprenger; Lorenz Trümper; Carsten Schlüter; Hans-Dieter Flad; Johannes Gerdes

A PCR method is described for determining the expression of multiple heterogeneous mRNAs from single cells. The total mRNA pool of a single selected cell is subjected to reverse transcription and subsequent tailing with poly(dA). This cDNA is preamplified by a sequence non-specific PCR protocol using oligo(dT)-containing primers. The single cell cDNA library obtained permits the analysis of virtually unlimited numbers of mRNA species per cell using sequence-specific PCR. This procedure of multiple mRNA analysis enables phenotyping of any cell for its mRNA composition and could be used to study the cytokine mRNA expression of individual human T cells ex vivo. The method should greatly facilitate the analysis of combinatorial expression of known genes in any cell.


Immunobiology | 1994

Detection of Mycobacterium leprae by Three-Primer PCR

Elvira Richter; Michael Duchrow; Carsten Schlüter; Margrit Hahn; Hans-D. Flad; Johannes Gerdes

Recently, polymerase chain reaction has been introduced for the species-specific assessment of Mycobacterium leprae (1). To avoid Southern blotting techniques using radioactively labelled oligonucleotide probes, the aim of this study was to establish a three primer-based single-step PCR technique. Using primers designed for this purpose we amplified a part of the gene encoding for the 16S ribosomal RNA of slowly growing mycobacteria. Due to the species-specific antisense primer a second, smaller fragment specific for M. leprae was amplified. Our results show that the employment of a second antisense primer in the PCR may be a substitution for Southern blot hybridization.


Immunobiology | 1994

Mycobacterium leprae DNA content, cellular and cytokine patterns in skin lesions of leprosy patients undergoing multidrug therapy (MDT).

Hans-D. Flad; Elvira Richter; Carsten Schlüter; Michael Duchrow; Jörg Arnoldi; Margrit Hahn; Wolfgang Grafvon Ballestrem; Arnaldo E. Alvarenga; Johannes Gerdes

Skin biopsies from untreated and MDT-treated patients were examined for infiltrating cells and cells producing the cytokines TNF-alpha, IFN-gamma, and IL-1 beta using immunohistochemistry. Biopsy specimens from untreated tuberculoid leprosy patients were characterized by the presence of cells producing TNF-alpha, IFN-gamma, and IL-1 beta and of subepidermal Langerhans cells. These cells were rarely found or completely absent in biopsies of untreated lepromatous leprosy patients, but tended to increase under MDT. In a short-term therapy trial for three months with brodimoprim, dapsone, and rifampicin, 12 patients were monitored by follow-up biopsies. Semiquantitative PCR for mycobacterial DNA revealed two groups of patients: one group in which mycobacterial DNA in follow-up biopsies remained constant and a second group in which a decrease of mycobacterial DNA during therapy was noted. Immunophenotyping in these follow-up biopsies revealed that in the latter group IFN-gamma-positive cells and Langerhans cells were present and gamma delta T cell receptor-positive cells tended to decrease during therapy. In contrast, in patients whose mycobacterial DNA did not change during therapy, these phenotypical manifestations were not observed. We therefore, conclude that assessment of mycobacterial DNA in combination with phenotyping of infiltrating cells and determination of cytokine patterns may be useful tools in establishing criteria for the effectiveness and duration of MDT in patients with leprosy.


Biochemical and Biophysical Research Communications | 1996

Human Dermal Fibroblasts Express Eotaxin: Molecular Cloning, mRNA Expression, and Identification of Eotaxin Sequence Variants

Joachim Bartels; Carsten Schlüter; Elvira Richter; Norio Noso; Reinhard Kulke; Enno Christophers; Jens-Michael Schröder


Journal of Investigative Dermatology | 1998

The CXC Receptor 2 Is Overexpressed in Psoriatic Epidermis

Reinhard Kulke; Erika Bornscheuer; Carsten Schlüter; Joachim Bartels; Joachim Röwert; Michael Sticherling; Enno Christophers


Biochemical and Biophysical Research Communications | 1997

Genomic Organization, Sequence, and Transcriptional Regulation of the Human Eotaxin Gene

Herbert Hein; Carsten Schlüter; Reinhard Kulke; Enno Christophers; Jens-Michael Schröder; Joachim Bartels


Rhinology | 1997

Increased eotaxin-mRNA expression in non-atopic and atopic nasal polyps: Comparison to RANTES and MCP-3 expression*

Joachim Bartels; Steffen Maune; Jens E. Meyer; Reinhard Kulke; Carsten Schlüter; Joachim Röwert; Enno Christophers; Jens M. Schröder


The Journal of Pathology | 1995

An improved method for the species-specific assessment of mycobacteria in routinely formalin-fixed and paraffin-embedded tissues

Elvira Richter; Carsten Schlüter; Michael Duchrow; Margrit Hahn; Sabine Rüsch-Gerdes; Jürgen Galle; Hans-D. Flad; Johannes Gerdes


Biochemical and Biophysical Research Communications | 1999

Genomic Organization, Sequence Analysis and Transcriptional Regulation of the Human MCP-4 Chemokine Gene (SCYA13) in Dermal Fibroblasts: A Comparison to Other Eosinophilic β-Chemokines

Herbert Hein; Carsten Schlüter; Reinhard Kulke; Enno Christophers; Jens-Michael Schröder; Joachim Bartels


Journal of Dermatological Science | 1998

Regulation of CXCR2 expression in human keratinocytes: Correlation with proliferation and differentiation

Carsten Schlüter; Reinhard Kulke; Joachim Bartels; Enno Christophers; J.M. Schroeder

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Johannes Gerdes

Free University of Berlin

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