Intranuclear post-transcriptional down-regulation responsible for loss of a keratin differentiation marker in tumour progression

Apparent loss of differentiation markers characterizes advanced malignant neoplasms. Post-transcriptional down-regulation of keratin message to levels undetectable with a partial cDNA probe to rat keratin K5 had been observed in anaplastic cells (T952/F7) derived from benign keratin-producing cells...

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Bibliographic Details
Published inAnticancer research Vol. 15; no. 5B; p. 2145
Main Authors Paine, M L, Gibbins, J R, Choi, J K, McDonald, D A, Manthey, A M, Walker, D M, Kefford, R F
Format Journal Article
LanguageEnglish
Published Greece 01.09.1995
Subjects
Animals
Base Sequence
Cell Differentiation
Cell Nucleus - metabolism
Down-Regulation
Gene Expression Regulation, Neoplastic
Humans
In Situ Hybridization
Introns
Keratins - genetics
Molecular Sequence Data
Neoplasms - genetics
Neoplasms - pathology
Polymerase Chain Reaction
Rats
RNA, Messenger - analysis
Tetradecanoylphorbol Acetate - pharmacology
Tumor Cells, Cultured
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Summary:Apparent loss of differentiation markers characterizes advanced malignant neoplasms. Post-transcriptional down-regulation of keratin message to levels undetectable with a partial cDNA probe to rat keratin K5 had been observed in anaplastic cells (T952/F7) derived from benign keratin-producing cells (A5P/B10) (1). The entire fifth introns of both the K5 and K6 genes were generated from rat genomic DNA by PCR to define expression of these closely related proteins. Sequencing of the PCR products revealed 84% homology in the K5 and K6 exon regions included, but absence of any homology in the introns. Active transcription of K5 could be demonstrated in the anaplastic cells with reverse transcription of nuclear RNA (RTn-PCR) by the presence of PCR-generated products confirmed by sequencing as unspliced and spliced transcripts of rat K5. In situ hybridization with ssDNA probes for the spliced message from this region of the K5 gene demonstrated a punctuate distribution in the cytoplasm of the benign cells and absence of any detectable message in the anaplastic derivatives, ssDNA probes for the unspliced transcript containing intron 5 and the same flanking exon sequences as the spliced probe detected transcription of hnRNA in the anaplastic cells as discrete signals confined to the nuclear compartment. These results show that failure to express mRNA for a differentiation marker in the cytoplasm of anaplastic cells can be due to a mechanism operating in the nuclear compartment after gene transcription and indicate that the mechanism functions shortly after splicing of the transcript.
ISSN:0250-7005