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Your search keyword '"Dworniczak B"' showing total 13 results
Start Over Author "Dworniczak B" Publisher wiley
13 results on '"Dworniczak B"'

1. Blood-based detection of RAS mutations to guide anti-EGFR therapy in colorectal cancer patients: concordance of results from circulating tumor DNA and tissue-based RAS testing

Author

Schmiegel, W, Scott, RJ, Dooley, S, Lewis, W, Meldrum, CJ, Pockney, P, Draganic, B, Smith, S, Hewitt, C, Philimore, H, Lucas, A, Shi, E, Namdarian, K, Chan, T, Acosta, D, Ping-Chang, S, Tannapfel, A, Reinacher-Schick, A, Uhl, W, Teschendorf, C, Wolters, H, Stern, J, Viebahn, R, Friess, H, Janssen, K-P, Nitsche, U, Slotta-Huspenina, J, Pohl, M, Vangala, D, Baraniskin, A, Dockhorn-Dworniczak, B, Hegewisch-Becker, S, Ronga, P, Edelstein, DL, Jones, FS, Hahn, S, Fox, SB, Schmiegel, W, Scott, RJ, Dooley, S, Lewis, W, Meldrum, CJ, Pockney, P, Draganic, B, Smith, S, Hewitt, C, Philimore, H, Lucas, A, Shi, E, Namdarian, K, Chan, T, Acosta, D, Ping-Chang, S, Tannapfel, A, Reinacher-Schick, A, Uhl, W, Teschendorf, C, Wolters, H, Stern, J, Viebahn, R, Friess, H, Janssen, K-P, Nitsche, U, Slotta-Huspenina, J, Pohl, M, Vangala, D, Baraniskin, A, Dockhorn-Dworniczak, B, Hegewisch-Becker, S, Ronga, P, Edelstein, DL, Jones, FS, Hahn, S, and Fox, SB

Abstract

An accurate blood-based RAS mutation assay to determine eligibility of metastatic colorectal cancer (mCRC) patients for anti-EGFR therapy would benefit clinical practice by better informing decisions to administer treatment independent of tissue availability. The objective of this study was to determine the level of concordance between plasma and tissue RAS mutation status in patients with mCRC to gauge whether blood-based RAS mutation testing is a viable alternative to standard-of-care RAS tumor testing. RAS testing was performed on plasma samples from newly diagnosed metastatic patients, or from recurrent mCRC patients using the highly sensitive digital PCR technology, BEAMing (beads, emulsions, amplification, and magnetics), and compared with DNA sequencing data of respective FFPE (formalin-fixed paraffin-embedded) tumor samples. Discordant tissue RAS results were re-examined by BEAMing, if possible. The prevalence of RAS mutations detected in plasma (51%) vs. tumor (53%) was similar, in accord with the known prevalence of RAS mutations observed in mCRC patient populations. The positive agreement between plasma and tumor RAS results was 90.4% (47/52), the negative agreement was 93.5% (43/46), and the overall agreement (concordance) was 91.8% (90/98). The high concordance of plasma and tissue results demonstrates that blood-based RAS mutation testing is a viable alternative to tissue-based RAS testing.

Published
2017

5. Reassignment of theEPB4·1gene to 1p36 and assessment of its involvement in neuroblastomas

Author

Huang, S., primary, Lichtenauer, U. D., additional, Pack, S., additional, Wang, C., additional, Kim, A. C., additional, Lutchman, M., additional, Koch, C. A., additional, Torres-Cruz, J., additional, Huang, S.-C., additional, Benz, E. J., additional, Christiansen, H., additional, Dockhorn-Dworniczak, B., additional, Poremba, C., additional, Vortmeyer, A. O., additional, Chishti, A. H., additional, and Zhuang, Z., additional

Published
2001
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12. Reassignment of the EPB4.1 gene to 1p36 and assessment of its involvement in neuroblastomas.

Author

Huang S, Lichtenauer UD, Pack S, Wang C, Kim AC, Lutchman M, Koch CA, Torres-Cruz J, Huang SC, Benz EJ Jr, Christiansen H, Dockhorn-Dworniczak B, Poremba C, Vortmeyer AO, Chishti AH, and Zhuang Z

Subjects
Alternative Splicing, Base Sequence, Chromosome Deletion, Chromosome Mapping, DNA Mutational Analysis, DNA, Complementary genetics, DNA, Neoplasm genetics, Gene Expression, Humans, In Situ Hybridization, Fluorescence, Membrane Proteins metabolism, Membranes metabolism, Mutation, Neuroblastoma metabolism, Protein Isoforms genetics, Tumor Cells, Cultured, Chromosomes, Human, Pair 1 genetics, Cytoskeletal Proteins, Membrane Proteins genetics, Neuroblastoma genetics, Neuropeptides
Abstract

Objectives: EPB4.1 has been previously mapped to human chromosome 1p33-p34.2. In contradiction to this chromosomal location, we have mapped EPB4.1-1p36 by using fluorescence in situ hybridization and radiation hybrid mapping. In neuroblastomas, deletions of the telomeric end of chromosome 1 (1p36) are the most common genetic aberration., Methods: We investigated whether genetic aberrations of EPB4.1 can be detected in some neuroblastomas by analyzing 72 tumours for EPB4.1 mutation, expression, and alternative splicing pattern. Furthermore, EPB4.1 protein from a neuroblastoma cell line was studied for its subcellular localization., Results: Sequence changes could be detected in 14 out of 72 neuroblastomas, including missense, silent, and intronic changes. Duplex RT-PCR analysis revealed a subset of 11 tumours expressing significantly low levels of EPB4.1. Significant EPB4.1 sequence changes that were detected included an exon 4 G/A missense mutation (amino acid: V/I) that was shown to be associated with absence of wild-type EPB4.1 expression (3 tumours), an exon 8 G/A missense mutation (V/M) (1 tumour), and an intronic sequence change that was shown to be associated with the presence of an aberrant transcript (1 tumour). Splicing pattern analysis revealed that all EPB4.1 transcripts from tumours exclude exon 3, a splicing pattern for generating the 135 kDa isoform. EPB4.1 cDNA cloned from a neuroblastoma cell line produced a 135-kDa protein with a cytoplasm/membrane localization., Conclusions: Out of 72 neuroblastomas we have identified 11 tumours with impaired EPB4.1 expression and 5 tumours with significant sequence changes. We also found that the 135 kDa isoform is the main EPB4.1 product in neuroblastoma. EPB4.1 cDNA from a neuroblastoma cell line produced a 135-kDa protein and displayed a cytoplasm/membrane localization in transfected cells.

Published
2001
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