A sensitive, single-tube assay to measure the enzymatic activities of influenza RNA polymerase and other poly(A) polymerases: application to kinetic and inhibitor analysis

doi:10.1093/nar/29.13.2691

This Article

	Full Text
	Print PDF (240K)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Email this article to a friend
	Similar articles in this journal
	Similar articles in ISI Web of Science
	Similar articles in PubMed
	Alert me to new issues of the journal
	Add to My Personal Archive
	Download to citation manager
	Search for citing articles in: ISI Web of Science (1)
	Request Permissions
	Commercial Re-use Guidelines for Open Access NAR Content

Google Scholar

	Articles by Hooker, L.
	Articles by Klumpp, K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Hooker, L.
	Articles by Klumpp, K.

Related Collections

	Enzyme assays
	Monitoring gene expression

Social Bookmarking

	What's this?

Nucleic Acids Research, 2001, Vol. 29, No. 13 2691-2698
© 2001 Oxford University Press

A sensitive, single-tube assay to measure the enzymatic activities of influenza RNA polymerase and other poly(A) polymerases: application to kinetic and inhibitor analysis

Lisa Hooker, Rebecca Strong, Ralph Adams, Balraj Handa¹, John H. Merrett¹, Joseph A. Martin¹ and Klaus Klumpp^* Department of Biology and ¹Department of Chemistry, Roche Discovery Welwyn, 40 Broadwater Road, Welwyn Garden City, Hertfordshire AL7 3AY, UK

We describe a fast and robust new assay format to measure poly(A)polymerase (PAP) activity in a microtiter plate format. Thenew assay principle uses only natural nucleotide triphosphatesand avoids a labour-intensive filtration step. A coupled enzymaticsystem combining PAP and reverse transcriptase forms the basisof the assay. The PAP generates a poly(A) tail on a RNA substrateand the reverse transcriptase is used to quantify the polyadenylatedRNA by extension of a biotinylated oligo-dT primer. We demonstratethe principle of the assay using influenza virus RNA polymeraseand yeast PAP as examples. A specific increase in the K_m valuefor ATP and the observation of burst kinetics in the polyadenylationdependent, but not in the polyadenylation independent, assaysuggest that a rate limiting step of influenza polymerase activityoccurs after transcription elongation. Yeast PAP was used tovalidate the assay as an example of a template independent PAP.The new yeast PAP assay was $~$ 100-fold more sensitive than theconventional TCA precipitation assay for yeast PAP, but thekinetic analysis of the PAP reaction gave similar results inboth assays. The two enzymes show important differences withrespect to inhibition by 3'-deoxy-ATP. Whereas the K_i valuefor 3'-deoxy-ATP (105–117 µM) is similar to theK_m value for ATP (186 µM) in the case of influenza RNApolymerase, the K_i value for 3'-deoxy-ATP (0.4–0.6 µM)is $~$ 100-fold lower than the K_m value for ATP (50 µM) inthe case of yeast PAP.

^* To whom correspondence should be addressed. Tel: +44 1707 361085;Fax: +44 1707 332053; Email: klaus.klumpp{at}roche.com

Add to CiteULike CiteULike Add to Connotea Connotea Add to Del.icio.us Del.icio.us What's this?

This article has been cited by other articles:

L. S. Chen and T. L. Sheppard
Chain Termination and Inhibition of Saccharomyces cerevisiae Poly(A) Polymerase by C-8-modified ATP Analogs
J. Biol. Chem., September 24, 2004; 279(39): 40405 - 40411.
[Abstract] [Full Text] [PDF]