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RESEARCH ARTICLE

A comparison of the excretion rate of endogenous purine derivatives in the urine of Bos indicus and Bos taurus steers

M. K. Bowen A B C , D. P. Poppi A , S. R. McLennan B and V. J. Doogan B
+ Author Affiliations
- Author Affiliations

A Schools of Animal Studies and Veterinary Science, University of Queensland, St Lucia, Qld 4072, Australia.

B Animal Science, Department of Primary Industries and Fisheries, Animal Research Institute, Moorooka, Qld 4105, Australia.

C Corresponding author. Email: maree.bowen@dpi.qld.gov.au

Australian Journal of Agricultural Research 57(2) 173-177 https://doi.org/10.1071/AR05182
Submitted: 25 May 2005  Accepted: 10 October 2005   Published: 24 February 2006

Abstract

Estimates of microbial crude protein (MCP) production by ruminants, using a method based on the excretion of purine derivatives in urine, require an estimate of the excretion of endogenous purine derivatives (PD) by the animal. Current methods allocate a single value to all cattle. An experiment was carried out to compare the endogenous PD excretion in Bos taurus and high-content B. indicus (hereafter, B. indicus) cattle. Five Holstein–Friesian (B. taurus) and 5 Brahman (> 75% B. indicus) steers (mean liveweight 326 ± 3.0 kg) were used in a fasting study. Steers were fed a low-quality buffel grass (Cenchrus ciliaris; 59.4 g crude protein/kg dry matter) hay at estimated maintenance requirements for 19 days, after which hay intake was incrementally reduced for 2 days and the steers were fasted for 7 days. The excretion of PD in urine was measured daily for the last 6 days of the fasting period and the mean represented the daily endogenous PD excretion. Excretion of endogenous PD in the urine of B. indicus steers was less than half that of the B. taurus steers (190 µmol/kg W0.75.day v. 414 µmol/kg W0.75.day; combined s.e. 37.2 µmol/kg W0.75.day; P < 0.001). It was concluded that the use of a single value for endogenous PD excretion is inappropriate for use in MCP estimations and that subspecies-specific values would improve precision.

Additional keywords: rumen microbial protein, cattle.


Acknowledgments

This study was mainly funded by the Department of Primary Industries and Fisheries, Queensland, which provided post-graduate support for M. K. Bowen. M. K. Bowen was also in receipt of an Australian Government Postgraduate Research Award. The analysis of purine derivatives by M. Nielsen and the technical assistance of ‘Mt Cotton’ staff are appreciated, as well as veterinary supervision of the cattle by J. Gibbs.


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