Edgar F. Garrett scite author profile

Two experiments were conducted 1) to validate a field protocol for the determination of ruminal pH and 2) to develop a strategy to interpret ruminal pH data from groups of cows. In the first experiment, ruminal fluid was collected from 30 lactating dairy cows. Ruminal fluid pH was 0.28 pH units lower for fluid collected by rumenocentesis than for fluid collected through a ruminal cannula. Concentrations of volatile fatty acids were correspondingly higher in samples collected by rumenocentesis. A portable pH meter capable of measuring pH of a very small volume of ruminal fluid yielded very similar pH readings as did a standard meter with a pH probe. Filtration or aspiration of ruminal fluid had no effect on pH. In the second experiment, a strategy was developed to use ruminal pH values from a subsample of cows to distinguish between groups fed either a low or higher forage diet. Groups could be distinguished using a cut point of 5.5 ruminal pH, a sample size of 12 cows, and a critical value of 3 or more cows below the cut point. This strategy had the lowest theoretical error rate for herds with either a high or low prevalence of cows with a low ruminal pH.

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A transcriptomal analysis of bovine oviductal epithelial cells collected during the follicular phase versus the luteal phase of the estrous cycle

Garrett

Walton

et al. 2015

Reprod Biol Endocrinol

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BackgroundReproductive success depends on a functional oviduct for gamete storage, maturation, fertilization, and early embryonic development. The ovarian-derived steroids estrogen and progesterone are key regulators of oviductal function. The objective of this study was to investigate luteal and follicular phase-specific oviductal epithelial cell function by using microarray-based transcriptional profiling, to increase our understanding of mRNAs regulating epithelial cell processes, and to identify novel genes and biochemical pathways that may be found to affect fertility in the future.MethodsSix normally cycling Angus heifers were assigned to either luteal phase (LP, n = 3) or follicular phase (FP, n = 3) treatment groups. Heifers in the LP group were killed between day 11 and 12 after estrus. Heifers in the FP group were treated with 25 mg PGF2α (Lutalyse, Pfizer, NY) at 8 pm on day 6 after estrus and killed 36 h later. Transcriptional profiling by microarray and confirmation of selected mRNAs by real-time RT-PCR analyses was performed using total RNA from epithelial cells isolated from sections of the ampulla and isthmus collected from LP and FP treatment groups. Differentially expressed genes were subjected to gene ontology classification and bioinformatic pathway analyses.ResultsStatistical one-way ANOVA using Benjamini-hochberg multiple testing correction for false discovery rate (FDR) and pairwise comparison of epithelial cells in the ampulla of FP versus LP groups revealed 972 and 597 transcripts up- and down-regulated, respectively (P < 0.05). Within epithelial cells of the isthmus in FP versus LP groups, 946 and 817 transcripts were up- and down-regulated, respectively (P < 0.05). Up-regulated genes from both ampulla and isthmus were found to be largely involved in cholesterol biosynthesis and cell cycle pathways, while down-regulated genes were found in numerous inflammatory response pathways.ConclusionsMicroarray-based transcriptional profiling revealed phase of the cycle-dependent changes in the expression of mRNA within the epithelium of the oviducts’ ampulla and isthmus.Electronic supplementary materialThe online version of this article (doi:10.1186/s12958-015-0077-1) contains supplementary material, which is available to authorized users.

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Detection, quantifications and pharmacokinetics of toltrazuril sulfone (Ponazuril^®) in cattle

Dirikolu

Yohn

Garrett

et al. 2009

Vet Pharm & Therapeutics

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Toltrazuril sulfone (Ponazuril) is a triazine-based anti-protozoal agent with highly specific actions against apicomplexan group of organisms, which are undergoing intensive investigation. Toltrazuril sulfone may have clinical application in the treatment of Neospora. caninum and other protozoal infections in cattle. To evaluate absorption, distribution, and elimination characteristics of toltrazuril sulfone in cattle, a sensitive validated quantitative high-pressure liquid chromatography method for toltrazuril sulfone in bovine biological fluids was developed. After a single oral dose of toltrazuril sulfone at 5 mg/kg (as 150 mg/g of Marquis; Bayer HealthCare, Shawnee Mission, KS, USA), samples from six cows showed good plasma concentrations of toltrazuril sulfone, which peaked at 4821 ng/mL +/- 916 (SD) at 48 h postadministration. Thereafter, plasma concentration declined to 1950 ng/mL +/- 184 (SD) at 192 h after administration with an average plasma elimination half-life of approximately 58 h. Following oral dose of toltrazuril sulfone, the observed peak plasma concentrations were in relatively close agreement ranging from the lowest 3925 ng/mL to the highest of 6285 ng/mL with the mean peak plasma concentration being 4821 ng/mL. This study shows that toltrazuril sulfone is relatively well absorbed after oral dose in cattle. These results are therefore entirely consistent with and support the reported clinical efficacy of toltrazuril sulfone in the treatment of experimentally induced clinical cases of N. caninum and other protozoal-mediated bovine diseases.

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Comparative analysis of four commercial on-farm culture methods to identify bacteria associated with clinical mastitis in dairy cattle

et al. 2018

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Several multiple-media culture systems have become commercially available for on-farm identification of mastitis-associated pathogens. However, the accuracy of these systems has not been thoroughly and independently validated against microbiological evaluations performed by referral laboratories. Therefore, the purpose of the present study was to evaluate the performance of commercially available culture plates (Accumast, Minnesota Easy System, SSGN and SSGNC Quad plates) to identify pathogens associated with clinical mastitis in dairy cows. Milk samples from the affected quarter with clinical mastitis were aerobically cultured with the on-farm culture systems and by two additional reference laboratories. Agreeing results from both standard laboratories were denoted as the reference standard (RS). Accuracy (Ac), sensitivity (Se), specificity (Sp), positive and negative predictive values (PPV and NPV, respectively) and Cohen’s kappa coefficient (k) of on-farm plates were determined based on the RS culture of 211 milk samples. All four plate-systems correctly identified ≥ 84.9% of milk samples with no bacterial growth. Accumast had greater values for all overall predictive factors (Ac, Se, Sp, PPV and NPV) and a substantial agreement (k = 0.79) with RS. The inter-rater agreements of Minnesota, SSGN, and SSGNC with RS were moderate (0.45 ≤ k ≤ 0.55). The effectiveness to categorize bacterial colonies at the genus and species was numerically different amongst the commercial plates. Our findings suggest that Accumast was the most accurate on-farm culture system for identification of mastitis-associated pathogens of the four systems included in the analysis.

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Partial Replacement of Forage with Nonforage Fiber Sources in Lactating Cow Diets. I. Performance and Health

Pereira¹,

Garrett²,

Oetzel³

et al. 1999

Journal of Dairy Science

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Edgar F. Garrett

Diagnostic Methods for the Detection of Subacute Ruminal Acidosis in Dairy Cows

A transcriptomal analysis of bovine oviductal epithelial cells collected during the follicular phase versus the luteal phase of the estrous cycle

Detection, quantifications and pharmacokinetics of toltrazuril sulfone (Ponazuril^®) in cattle

Comparative analysis of four commercial on-farm culture methods to identify bacteria associated with clinical mastitis in dairy cattle

Partial Replacement of Forage with Nonforage Fiber Sources in Lactating Cow Diets. I. Performance and Health

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Edgar F. Garrett

Diagnostic Methods for the Detection of Subacute Ruminal Acidosis in Dairy Cows

A transcriptomal analysis of bovine oviductal epithelial cells collected during the follicular phase versus the luteal phase of the estrous cycle

Detection, quantifications and pharmacokinetics of toltrazuril sulfone (Ponazuril®) in cattle

Comparative analysis of four commercial on-farm culture methods to identify bacteria associated with clinical mastitis in dairy cattle

Partial Replacement of Forage with Nonforage Fiber Sources in Lactating Cow Diets. I. Performance and Health

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Product

Resources

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Detection, quantifications and pharmacokinetics of toltrazuril sulfone (Ponazuril^®) in cattle