Four healthy nonpregnant, nonlactat

Four healthy nonpregnant, nonlactating, ovariectomized Holstein cows (age 6.2 to 8.2 yr; body weight 610 + 63 kg) were used in this study. A bilateral ovariectomy was performed in each cow by lateral laparotomy at least 3 mo prior to the experiment to exclude the effects of gonadal steroid hormones. The cows were housed separately and loose tied at least 1 week prior to the start of the experiment. The cows were fed 5 kg of grass hay and 0.5 kg of concentrate twice
daily and had free access to tap water. One intravenous catheter was inserted into each jugular vein 1 day prior to the ACTH infusion to alleviate the stress associated with the infusion and blood collection. An extension tube was connected to the catheter for blood collection and fixed to the halter.
The dose of ACTH was based on previous studies [7,8].
Synthetic ACTH (0.5 mg, Cortrosyn, Daiichi-Sankyo,
Tokyo, Japan) was dissolved in 2 L of isotonic NaCl
solution. The experiment was performed according to a
2
2 crossover design. In brief, cows were infused for
12 h with either ACTH solution at a rate of 41.67
g/h
or isotonic NaCl solution as a corresponding control,
and 1 wk later these processes were carried out again,
but with infusion of the solution that the animal had not
yet received. Blood samples were collected before the
start of infusion (0 h; baseline) and at 6, 12, 15, 18, 21,
24, 36, 48, 60, and 72 h after the start of infusion using
heparinized tubes (BD Vacutainer, Becton, Dickson
and Company, Plymouth, UK). The blood samples
were placed on ice immediately and centrifuged
(1,000g, 15 min) within 10 min. Separated plasma was
stored at 50°C until analysis. This study protocol was
approved by the Iwate University Laboratory Animal
Care and Use Committee.
All biochemical parameters were determined in duplicate.
Plasma cortisol concentrations were measured
by radioimmunoassay (cortisol RIA, TFB Ltd, Tokyo,
Japan; intra-assay coefficient of variance 3.6  0.4%;
interassay coefficient of variance 2.8  0.3%). Plasma
glucose (hexokinase method), Ca (ortho-cresolphthalein
complexone method), Pi (purine nucleoside phosphorylase,
xanthine dehydrogenase method), and magnesium
(Mg, isocitrate dehydrogenase method) were
measured using an Accute TBA-40FR AutoAnalyzer
(Toshiba, Tokyo, Japan) and commercial test kits.
Plasma activity oftartrate-resistant acid phosphatase
isoform 5b (TRAP5b) and plasma concentration of hydroxyproline
(HYP), the bone resorption markers, was
determined fluorometrically [9] and spectrophotometrically
[10], respectively. The activity of bone-specific
alkaline phosphatase (BALP), a bone formation marker,
was measured spectrophotometrically using a LabAssay
ALP kit (Wako Pure Chemical Industries Ltd,
Osaka, Japan) and the heat-inactivation method (56°C,
15 min) [11].
Numerical data are presented as the mean  SD.
After Kolmogorov–Smirnov normality testing, parametric
data were analyzed by one-way repeated-measures
analysis of variance and the Holm–Sidak post hoc
test to compare the changes in each parameter for each
group. Nonnormally distributed data were analyzed by
one-way repeated-measures analysis of variance on
rank, followed by Dunn’s test. Student’s t-test or Mann–
Whitney U test was performed after the normality
test to compare groups at the same time point. Significance
was set at P  0.05. Analyses were performed