weighed on to a filter paper and pl

weighed on to a filter paper and placed manually in the
rumen mat via the rumen cannula on day 8 through day 16.
The marker was placed in the rumen three times per day at
0800, 1500 and 2100 h. Feces were collected from days 13
to 17 by rectal sampling failing voluntary defecation in a
design that equally represented the 96-h collection period as
well as the 24 h day (Khorasani et al., 1996). The sampling
times were 0730, 1930, 0430, 1630, 0130, 1330, 1030 and
2230 h. At each sampling time, 200 g of feces were collected
from each cow and stored at 2208C until analysis. Samples
were pooled by cow by period.
Rumen fluid was sampled 12 times over a 24-h period
beginning on day 18. Samples were obtained at 0730, 0810,
0830, 0900, 0930, 1000, 1200, 1400, 1600, 1800, 0200 and
0600 h. Rumen fluid was collected using a stainless steel
strainer attached to a plastic tube that was inserted in the
dorsal, middle and ventral sections of the rumen to obtain a
representative sample (100 ml from each location). The
liquid was extracted by applying vacuum to the end of the
tube with a syringe (Khorasani and Kennelly, 2001). One 4ml
aliquot for volatile fatty acid (VFA) analysis was placed in a
test tube containing 1ml 25% H3PO4 and stored at 2208C
until analyzed. A second aliquot was placed in another test
tube and stored at 2208C for ammonia–N analysis.
Rumen pH was continuously measured from days 12 to 15
using indwelling rumen pH probes as described by Penner
et al. (2006). Ruminal pH readings were taken every 30 s and
averaged every 60 s and were summarized daily for each