Your search keyword '"Elizabeth J. Payne"' showing total 2 results

1. RNA-seq reveals more consistent reference genes for gene expression studies in human non-melanoma skin cancers

Author

Van L.T. Hoang, Lisa N. Tom, Xiu-Cheng Quek, Jean-Marie Tan, Elizabeth J. Payne, Lynlee L. Lin, Sudipta Sinnya, Anthony P. Raphael, Duncan Lambie, Ian H. Frazer, Marcel E. Dinger, H. Peter Soyer, and Tarl W. Prow

Subjects

RNA-seq, Reference gene, qPCR, Non-melanoma skin cancer, Medicine, Biology (General), QH301-705.5

Abstract

Identification of appropriate reference genes (RGs) is critical to accurate data interpretation in quantitative real-time PCR (qPCR) experiments. In this study, we have utilised next generation RNA sequencing (RNA-seq) to analyse the transcriptome of a panel of non-melanoma skin cancer lesions, identifying genes that are consistently expressed across all samples. Genes encoding ribosomal proteins were amongst the most stable in this dataset. Validation of this RNA-seq data was examined using qPCR to confirm the suitability of a set of highly stable genes for use as qPCR RGs. These genes will provide a valuable resource for the normalisation of qPCR data for the analysis of non-melanoma skin cancer.

Published

2017

2. Loss of PKR activity in chronic lymphocytic leukemia.

Author

Su Ing Hii, Lani Hardy, Tania Crough, Elizabeth J. Payne, Karen Grimmett, Devinder Gill, and Nigel A.J. McMillan

Subjects

PROTEIN kinases, LEUKEMIA genetics, B cells, P53 antioncogene

Abstract

There are a number of observations that suggest the dsRNA-activated protein kinase, PKR, may play an active role in formation and maintenance of leukemia, including nonrandom chromosomal deletions in acute leukemia as well as truncations and deletions of the PKR gene in some leukemia cell lines. However, there is little direct evidence from patient material that this is so. Here we show that full-length PKR is present but not active in 21 of 28 patient samples from B-cell chronic lymphocytic leukemia (B-CLL). PKR from these patients was unable to auto-activate or phosphorylate substrates but was able to bind dsRNA. Furthermore, the lack of PKR activation was not due to differing levels of the PKR activator, PACT nor of the PKR inhibitor, p58IPK. We compared PKR status with clinical parameters and disease staging. No differences were found between the 2 groups in terms of staging (modified Rai or Binet), age, CD38 status, p53 status, 11q23 deletion status or CEP12 deletion status. However, there was a significant correlation between deletion in 13q14.3 and lack of PKR activity. We show that B-CLL cells appear to contain a soluble inhibitor of PKR, as lysates from cells lacking PKR activity were able to inhibit exogenous PKR in mixing experiments. Finally, we show suppression of PKR activity was still present following ultrafilitration through a 10,000 Da cutoff filter but was lost upon extraction with phenol/chloroform or by high salt washing. This data suggests loss of PKR activity may contribute to the formation and/or maintenance of CLL. © 2004 Wiley-Liss, Inc. [ABSTRACT FROM AUTHOR]

Published

2004