Activation of TRK Genes in Ewingʼs Sarcoma Trk A Receptor Expression Linked to Neural Differentiation

6533b86cfe1ef96bd12c8cb5

RESEARCH PRODUCT

Activation of TRK Genes in Ewingʼs Sarcoma Trk A Receptor Expression Linked to Neural Differentiation

Antonio Pellín Enrique Nogueira Antonio Llombart-bosch Samuel Navarro

subject

animal structures Receptor expression Receptors Nerve Growth Factor Sarcoma Ewing Biology Pathology and Forensic Medicine Mice Proto-Oncogene Proteins medicine Animals Neuroectodermal Tumors Primitive Receptor trkC Receptor trkA Receptor Receptor Ciliary Neurotrophic Factor Molecular Biology Neurons Membrane Proteins Receptor Protein-Tyrosine Kinases Ewing's sarcoma Cell Differentiation Cell Biology Protein-Tyrosine Kinases medicine.disease Molecular biology Gene Expression Regulation Neoplastic enzymes and coenzymes (carbohydrates)nervous system Trk receptor Primitive neuroectodermal tumor embryonic structures Immunohistochemistry Sarcoma Immunostaining

description

Trk receptors have been identified by immunohistochemical methods in primitive neuroectodermal tumor (PNET)/Ewing's sarcoma (ES). However, the presence of different members of the Trk family of receptors in PNET/ES has not been specified. We have examined whether Trk A, B, and C receptors are specifically expressed in ES both with and without features of neural differentiation. Ten ES tumors (five primary tumors of bone and five extraosseous tumors transplanted into nude mice) were investigated for expression of Trk receptors by immunohistochemistry and reverse transcription-polymerase chain reaction. One primary ES and the five grafted ES tumors exhibited signs of neural differentiation; the remaining four primaries were undifferentiated ES. Other tumor types were analyzed as controls; they included three neuroblastomas (NB), two lymphomas, and single cases of pheochromocytoma (PHEO), schwannoma (SCHW), osteosarcoma, and carcinoma of breast, colon, and kidney. Trk receptors were detected in paraffin-embedded tumor tissue sections by means of a pan-Trk polyclonal antibody raised against the 14 carboxy-terminal residues of gp140trk, and trk A, B, and C transcripts were specifically detected by polymerase chain reaction-based amplification on cDNAs derived from tumor RNA with MuLV reverse transcriptase. Reactivity to the pan-Trk antibody was exhibited by six ES tumors, the three NBs, and the single PHEO and SCHW cases; immunoreactivity was restricted to differentiated tumors, in the case of ES. Tumor types positive for immunostaining were also distinguished by containing transcripts of TRK genes. However, the trk A, B, and C expression pattern of ES differed from that of NBs, PHEO, and SCHW. Transcripts of trk A, B, and C were detected in seven, four, and one case of ES, respectively, and in five, two, and five cases of NB, PHEO, and SCHW, respectively. Interestingly, all differentiated ES tumors contained trk A transcripts. Tumors of neuroectodermal phenotype and/or derivation were thus characterized by a distinct consensus expression pattern: trk A+/B-/C+ for differentiated ES and trk A+/B-/C+ for NB-PHEO-SCHW. These results indicate that the TRK gene family is frequently activated in ES; they also suggest that Trk A receptor is a feature of ES with neural differentiation, whereas Trk B and C receptors seem to be present in undifferentiated ES.

year	journal	country	edition	language
1997-02-01	Diagnostic Molecular Pathology

https://doi.org/10.1097/00019606-199702000-00003