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ORIGINAL RESEARCH article

Front. Genet., 29 March 2012
Sec. Livestock Genomics

Evaluation of Bovine chemerin (RARRES2) Gene Variation on Beef Cattle Production Traits1


      Amanda K. Lindholm-Perry* Amanda K. Lindholm-Perry*Larry A. Kuehn Larry A. Kuehn
      Lea A. Rempel Lea A. Rempel
      Timothy P. L. Smith Timothy P. L. Smith
      Robert A. Cushman Robert A. Cushman
      Tara G. McDaneld Tara G. McDaneld
      Tommy L. Wheeler Tommy L. Wheeler
      Steven D. Shackelford Steven D. Shackelford
      David A. King David A. KingHarvey C. Freetly
   Harvey C. Freetly
  • U.S. Meat Animal Research Center, Agricultural Research Service, United States Department of Agriculture, Clay Center, NE, USA2

A previous study in cattle based on >48,000 markers identified markers on chromosome 4 near the chemerin gene associated with average daily feed intake (ADFI) in steers (P < 0.008). Chemerin is an adipokine associated with obesity and metabolic syndrome in humans, representing a strong candidate gene potentially underlying the observed association. To evaluate whether the bovine chemerin gene is involved in feed intake, 16 markers within and around the gene were tested for association in the same resource population. Eleven were nominally significant for ADFI (P < 0.05) and two were significant after Bonferroni correction. Two and five SNP in this region were nominally significant for the related traits of average daily gain (ADG) and residual feed intake (RFI), respectively. All markers were evaluated for effects on meat quality and carcass phenotypes. Many of the markers associated with ADFI were associated with hot carcass weight (HCW), adjusted fat thickness (AFT), and marbling (P < 0.05). Marker alleles that were associated with lower ADFI were also associated with lower HCW, AFT, and marbling. Markers associated with ADFI were genotyped in a validation population of steers representing 14 breeds to determine predictive merit across populations. No consistent relationships for ADFI were detected. To determine whether cattle feed intake or growth phenotypes might be related to chemerin transcript abundance, the expression of chemerin was evaluated in adipose of 114 heifers that were siblings of the steers in the discovery population. Relative chemerin transcript abundance was not correlated with ADFI, ADG, or RFI, but associations with body condition score and yearling weight were observed. We conclude that variation in the chemerin gene may underlie observed association in the resource population, but that additional research is required to determine if this variation is widespread among breeds and to develop robust markers with predictive merit across breeds.

Introduction

Beef cattle producers could increase profitability by selecting for animals with increased feed efficiency, and genetic markers for animals with superior performance may facilitate selection. Average daily feed intake (ADFI), average daily gain (ADG) and residual feed intake (RFI) are all heritable traits (h2 = 0.24–0.57; Snelling et al., 2011), and can be altered with genetic selection. Considering the high cost of feed, even small changes in the amount of feed that cattle consume could equate to significant cost savings for producers.

In a previous genome-wide association study, four markers from the Illumina BovineSNP50 BeadChip mapping to bovine chromosome 4 (BTA4) between 113.3 and 113.6 Mb (UMD 3.1, genome assembly, Zimin et al., 2009) were nominally significant (P ≤ 0.008) for ADFI in a USMARC population of crossbred steers (Snelling et al., 2011). The genes residing within this region included: 10 transfer RNA genes, three zinc finger genes involved in DNA and metal ion binding, KRAB-A domain containing 1 gene, the SCO-spondin homolog gene, ATPase, H+ transporting V0 subunit e2, leucine rich repeat containing 61, chromosome 4 open reading frame, human C7orf29 (C4H7orf29) gene, and the chemerin (RARRES2) gene.

The adipokine, chemerin, also known as retinoic acid receptor responder 2 (RARRES2) or tazarotene-induced gene 2 protein (TIG2), is located within this region on BTA4 at 113.5 Mb, and is a cytokine produced by adipose tissue. Adipokines are involved in adipogenesis and inflammation responses via autocrine and paracrine actions (Coppack, 2001; Wisse, 2004; Rhee, 2011). Chemerin is highly expressed in adipocytes and its receptor (CMKLR1, also known as ChemR23) is expressed in immune cells and adipose tissue (Goralski et al., 2007). Circulating levels of chemerin have been associated with symptoms of metabolic syndrome in humans including; body mass index (BMI), fasting serum insulin, triglycerides, and HDL cholesterol (Bozaoglu et al., 2007, 2009), making it an attractive functional candidate gene for feed intake in beef cattle.

Other adipokines have previously been associated with feed intake and efficiency. Higher serum levels of leptin, an adipose derived hormone, have been correlated with higher dry matter intake (DMI), RFI and partial efficiency of growth in beef steers (Nkrumah et al., 2007). Circulating levels and mRNA expression levels of adiponectin have also been implicated in rats with a diet-induced obesity phenotype (Pérez-Encharri et al., 2005).

The purpose of this study was to evaluate polymorphisms within the adipokine, chemerin, as a source of phenotypic variation in ADFI in a U.S. Meat Animal Research Center (USMARC) population of cattle. In addition, we evaluated the relative gene expression levels of chemerin for association with cattle growth, weight, and feed intake.

Materials and Methods

Animals

The USMARC Animal Care and Use Committee reviewed and approved all animal procedures. The procedures for handling the cattle complied with the Guide for the Care and Use of Agricultural Animals in Agricultural Research and Teaching (FASS, 1999).

Crossbred Steers (Discovery Population) and Heifers (Gene Expression)

The breeding scheme for the animals in the SNP discovery population (n = 1,066) and the heifers (n = 114) in this study has been described by Snelling et al. (2011). Briefly, purebred Angus, Hereford, Simmental, Limousin, Charolais, Gelbvieh, and Red Angus sires were bred to composite MARC III (1/4 Angus, 1/4 Hereford, 1/4 Pinzgauer, 1/4 Red Poll), Angus or Hereford cows by artificial insemination to produce F1 animals, born in 1999, 2000, and 2001. Female F1 and the 2001-born F1 males (Angus, Hereford dams only) were kept for breeding, and mated in multiple-sire pastures to produce 2-, 3-, and 4-breed cross progeny designated yes. The yes calves were born to 3-year-old and older dams in March through May from 2003 to 2007. Male calves were castrated within 24 h after birth. Calves were weaned in September at approximately 165 day of age (Snelling et al., 2011). Animals were screened and excluded for medical or health issues that may have affected either feed intake or gain phenotypes.

Validation Population

Validation animals (n = 406) were selected from progeny in the USMARC continuous Germplasm Evaluation Program (Kuehn et al., 2008). These animals were part of a breeding program to develop purebred cattle of each of the 14 breeds. In addition to the seven breeds mentioned above, this population also included Braunvieh, Shorthorn, Brahman, Maine Anjou, Santa Gertrudis, Salers, and Chi-Angus. Sires of each of these 14 breeds were mated to female descendents of cattle in the discovery population; none of the sires of the discovery population steers were sires of the validation animals. Approximately 60% of the validation animals were half-bloods sired by these seven new breeds and 40% were half- or three-quarter-bloods from the original seven breeds. Progeny were produced in three breeding seasons (Fall 2007, Spring 2008, and Fall 2008). Animals (n = 29) were removed from the analysis for chronic diagnoses (e.g., pneumonia, foot-rot, bloat).

Feed Efficiency Phenotypes

Calves were trained on the test ration as described in Snelling et al. (2011). Briefly, beginning at 276 ± 15 day of age, individual feed intake measurements were acquired with Calan Broadbent Feeding Systems (American-Calan-Broadbent, Northwood, NH, USA). Animals were given feed at 0800 h and had ad libitum access to the feed. The dry matter mixed ration included 82.0% dry rolled corn, 10.6% ground alfalfa hay, 5.66% soybean meal, 1.25% limestone, 0.4% urea, 0.06% salt, 0.007% trace minerals, 0.008% Vitamins A, D, and E, and 0.015% Rumensin 80. Feed refusals were obtained each week.

A description of feed efficiency phenotypes for yes steers and heifers can be found in Snelling et al. (2011). The phenotypes were collected as follows: DMI was equal to cumulative DMI for the 140-day-feeding period. ADFI is the average daily DMI (DMI/140). Individual animal quadratic regressions were fitted for body weight on time, and gain was calculated as the difference of BW predicted at 140 day and the intercept (Rolfe et al., 2011). ADG is the calculation for gain divided by days on feed. Predicted DMI was computed from the regression of DMI on 140 day gain and day 70 mid-test BW75. RFI was calculated as the difference between observed DMI and predicted DMI (Snelling et al., 2011).

The steers used for the validation study were fed for either 84 or 148 day at 302 ± 73 day of age. Feed intake for those fed for 84 day was measured using an Insentec system (Marknesse, The Netherlands). Diets were similar to that used in the discovery population. DMI was equal to the total DMI consumed for either the 84- or 148-day period and averaged to a daily basis (ADFI). A linear regression was used to predict BW in steers fed for 84 day and a quadratic equation was used to predict BW in steers fed for 140 day. ADG for both groups were calculated for the respective feeding periods as described in the discovery and heifer populations above.

Meat Quality and Carcass Phenotypes

The yes steers were serially harvested at a commercial processing plant as described by King et al. (2010) at 423 ± 66 day of age. USDA yield and quality grade data were provided by trained USMARC personnel after 36 h in the cooler at 0°C. Wholesale ribs were obtained as described by King et al. (2010). A posterior section of the ribeye was frozen at 14-d postmortem and a 2.54-cm thick steak was cut from the 11th rib region. For slice shear force (SSF), steaks were thawed at 5°C for 24 h, then cooked on a conveyor electric belt grill to a final internal temperature of 71°C as described by Wheeler et al. (2010). SSF was determined as described by Shackelford et al. (1999).

Cattle Body Condition Score

Body condition scores were obtained for yes heifers. Body condition scoring is conducted on a 9-point scale to describe the overall fatness of an animal (NRC, 1996). A BCS of 1 describes an emaciated animal with a body fat percent of ≤3.77. Five is an average BCS with body fat of 18.89% and a score of 9 describes a very fat animal with a body fat of ≥33.91% (NRC, 1996). Body condition scoring on yes heifers was performed at 530 ± 13 day of age.

Identification of SNP Markers in Chemerin (RARRES2)

Steers (n = 24) from the discovery population with extreme ADG or ADFI phenotypic and of different sire lines were selected for the SNP identification population. Twelve steers with low ADG or ADFI values and 12 steers with high ADG or ADFI phenotypes were chosen. Breeds were broadly represented in the animals with high and low phenotypes. Animals were screened and excluded for medical or health issues that may have affected either feed intake or gain phenotypes. Whole blood or buffy coats were collected from the steers for genomic DNA isolation.

Primer pairs to amplify the exonic and intronic boundaries of the chemerin gene from genomic DNA were designed using Primer3 (Rozen and Skaletsky, 2000). DNA sequences used as templates for primer design were obtained from the chromosome 4 Btau4.0 assembly. Oligonucleotide primers were synthesized by IDT (Integrated DNA Technologies, Coralville, IA, USA). PCR was performed in a DNA engine Dyad® peltier thermal cycler (Bio-Rad, Hercules, CA, USA). PCR reactions included 0.25 U Hot Star Taq polymerase (Qiagen, Valencia, CA, USA); 1× supplied buffer; 1.5 mM MgCl2; 80 μM dNTPs; 0.33 μM each primer; and 25 ng genomic DNA in 12 μl reactions. A portion of the PCR reaction (3 μl) was electrophoresed on 2% agarose gels to determine quality of amplification. The remainder was treated with 0.1 U exonuclease I (USB, Cleveland, OH, USA) and prepared for sequencing. Sequencing reactions were precipitated with 70% isopropanol and sequenced on an ABI 3730 sequencer (Applied Biosystems, Foster City, CA, USA). Bases were called with Phred and assembled into contigs with Phrap. Polymorphisms were identified using Polyphred and assessed using Consed4.

Genotyping Analysis

Multiplex assays for the Sequenom MASSARRAY® instrument were designed with the MASSARRAY® Assay Design 3.0 software (Sequenom, San Diego, CA, USA). Assays were designed to include 16 SNPs in and around chemerin from 113.54 to 113.62 Mb. Each amplification primer contained a 10-base tag to yield amplification products with different masses. Amplicon lengths were between 90 and 120 bp. Reaction conditions were performed as recommended by Sequenom. A total of 1,066 animals with DMI and ADG phenotypes and their sires (n = 71) were genotyped. The genotyping panel was redesigned to be a single multiplex assay for chemerin SNP for the validation and heifer populations. This panel included 12 SNP genotyped on the discovery population.

Statistical Analyses

The program MTDFREML (Boldman et al., 1995) was used to analyze markers for significant associations. Twin animals and cross-fostered animals were excluded from the analysis. The data were analyzed using an animal model that included the fixed effects of year and barn. Covariates of age and heterosis were also included. Calf and dam breed compositions were modeled with covariates for proportions Angus, Hereford, Simmental, Limousin, Charolais, Gelbvieh, Red Angus, and MARC III. Covariates for expected calf heterosis were computed from parental breed composition. SNP were fitted separately in the association model. Polygenic and breed effects were included to reduce the effects of family structure on breed- and family specific alleles (Kuehn et al., 2007; Goddard and Hayes, 2009). Variance components for polygenic effects and error were estimated using MTDFREML (Boldman et al., 1995). Nominal significance values were computed. Analyses of significant SNP in the validation population followed the same model definition.

RNA Isolation and Gene Expression

Adipose tissue was collected from yes heifers that were full or half siblings of the yes steers in the discovery population at 360 ± 40 day of age. Evaluation of BCS occurred at approximately 5 months after the adipose tissue collection. After lidocaine injection, subcutaneous adipose tissue was surgically removed from 450 heifers from a small incision placed roughly 10 cm down from the tailhead and immediately stored at −80°C until RNA extractions were performed. Total RNA was isolated from 50 to 100 mg of adipose tissue from a random sampling of 150 heifers using the RNeasy Lipid Kit (Qiagen, Valencia, CA, USA) according to the manufacturer’s instructions. Total RNA was quantified with a NanoDrop 8000 spectrophotometer (Wilmington, DE, USA). RNA (2 μg) was reverse transcribed using 0.5 μg ReadyMade random hexamer primers (Integrated DNA Technologies, Coralville, IA, USA) and M-MLV reverse transcriptase (Promega, Madison, WI, USA) according to the manufacturers protocol.

Primers used to amplify chemerin from cDNA were located in exons 2 and 3. Chemerin forward primer sequence was 5′-GGAGGAGTTCCACAAGCATC-3′ and the reverse primer sequence was 5′-CCAGTCTTTCTTCCGACAGC-3′. The reference or internal control gene protein kinase C inhibitor protein 1, also known as tyrosine 3-monooxygenase/tryptophan 5-monooxygenase activation protein, gamma polypeptide (YWHAG) forward primer sequence was 5′-GCGAGACCCAGTATGAGAGC-3′ and the reverse primer sequence was 5′-AAGGGCCAGGCCTAATCTAA-3′.

Real-time PCR was performed with 1× QuantiTect SYBR Green PCR Master Mix (Qiagen), 1 μl of 50 ng/μl cDNA template and 0.48 μM each primer. The PCR reaction was performed at 95°C for 5 min followed by 41 cycles at 95°C for 10 s, 58°C for 20 s, and 80°C for 1 s with a final melting curve from 78 to 95°C on a MJ PTC-200 with a Chromo-4 detector (MJ Research, Watertown, MA, USA). A pooled control sample was amplified with both primers sets on each plate. The threshold cycle (Ct) for chemerin and YWHAG from each sample was determined and used to calculate the ΔΔCt using the reference pooled cDNA samples. The fold difference between samples was obtained using the 2−ΔΔCt method (Livak and Schmittgen, 2001).

Gene Expression Data Analysis

Gene expression data using the comparative Ct method (ΔΔCt; Livak and Schmittgen, 2001) was analyzed for correlation with phenotypes using PROC CORR with SAS 9.2 (Cary, NC, USA) and MTDFREML. The ΔΔCt was chosen as the measure of expression because a reference pooled sample was used for normalization. The ΔΔCt units of expression displayed a normal distribution of values, low skewness (−0.05) and low kurtosis (−0.5). Gene expression data were analyzed for association with genotypes using MTDFREML. Fixed effects included birth year and date the tissue biopsy was performed. Covariates included gene expression plate, percent dam breed, breed percentage of each animal, and heterosis. Expression was also included as a covariate in phenotypic models for BCS and yearling weight adjusted to 365 day to detect the effect of higher expression of chemerin on each trait.

Linkage Disequilibrium Analysis

Linkage disequilibrium (LD; r2) was defined for the 16 SNP on chromosome 4 using Haploview 4.0 software (Barrett et al., 2005)5. Blocks of LD were based on pairwise LD values. Haploview settings were as follows: the exclusion of animals with >50% missing genotypes, ignoring pairwise comparisons of markers >500 kb apart, the percentage of genotypes ≤50% and minimum minor allele frequency of 0.001.

Results

Chemerin Marker Identification and Associations (Discovery Population)

To identify SNP in chemerin that may potentially be involved in cattle feed intake and growth variation, portions of the gene were sequenced in animals with extreme phenotypes. Four intronic SNP were identified (Table 1) and two of these were easily multiplexed into Sequenom iPLEX genotyping assays. Fourteen additional publicly available SNP located up- and down-stream of the chemerin gene from 113.54–113.62 Mb were also included in the genotyping assays (Table 2).

TABLE 1
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Table 1. SNP identified in chemerin in USMARC steers with extreme ADFI and ADG phenotypes.

TABLE 2
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Table 2. Markers on bovine chromosome 4 used to genotype the discovery population of steers.

Of the 16 SNP genotyped in the discovery population, 11 were nominally significant for ADFI (P ≤ 0.05); of which, two were significant for ADG (P ≤ 0.03) and five were significant for RFI (P ≤ 0.04; Table 3). One marker, 77244_529, located within intron 4 of the chemerin gene, was significant for all three phenotypes. After Bonferroni correction for multiple testing to account for testing 16 SNPs (P-value = 0.003; alpha = 0.05/16), three of the SNP (BTB-00210449, 77244_529, and BFGL-NGS-19480) remained significant for ADFI (P ≤ 0.05; Table 3). These three markers are in low LD with each other (r2 ≤ 0.32; data not shown).

TABLE 3
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Table 3. Marker associations and estimated effects for ADFI, ADG and RFI in the discovery population of steers.

These markers were also analyzed for their effects on meat quality and carcass traits (Table 4). Several of these markers were significantly associated with adjusted fat thickness (AFT), hot carcass weight (HCW) and marbling score (nominal P ≤ 0.05), but none were associated with ribeye area (REA) or SSF.

TABLE 4
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Table 4. Association and effects of markers on BTA4 with meat quality and carcass traits in the discovery population of steers.

Marker Validation

A validation of 12 of the markers tested in the discovery population (eight significantly associated with ADFI) was performed on a crossbred validation population of steers (n = 406) that included seven additional breeds of beef cattle (Table 5). Of the markers genotyped, none were validated with feed intake and gain in this population.

TABLE 5
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Table 5. Association and effect of markers within and near chemerin on the validation population of steers.

Chemerin Gene Expression

Chemerin gene expression (ΔΔCt) was examined in adipose tissue collected from heifers related to the discovery population of steers (Table 6). Chemerin gene expression was correlated with BCS (r = 0.29; P = 0.0015) and 365 day adjusted yearling weight (r = 0.20; P = 0.03; Table 6). There was slight, but not significant (P ≤ 0.16), correlation between chemerin gene expression and DMI and RFI (r = 0.14 and 0.13, respectively; Table 6). We also analyzed gene expression with BCS using the statistical analysis program MTDFREML. The estimated effect of expression on BCS was 1 unit of ΔΔCt per 0.142 units increase in BCS (P = 0.004).

TABLE 6
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Table 6. Correlation coefficients for heifer phenotypes.

Chemerin gene expression and BCS were also evaluated for association with the markers located within and surrounding chemerin (data not shown). None of the markers were significant for chemerin gene expression or BCS.

Discussion

Several markers on the Illumina BovineSNP50 BeadChip located near the chemerin gene on BTA4 were previously found to be associated with ADFI (P = 0.001–0.008) in the discovery population of steers (Snelling et al., 2011). In this study, we have further investigated chemerin SNP and gene expression as a source of feed intake phenotypic variation. These are the first studies that we are aware of associating genetic markers in and near the chemerin gene with feed intake variation in animals. The SNP presented in this study, along with those in this region on the BeadChip, may be useful for genetic selection of animals with superior phenotypes in multiple breeds of beef cattle. Moreover, we showed that variation in body condition score (BCS), a measure similar to BMI in humans, was positively correlated with chemerin gene expression.

The genetic markers analyzed in the discovery steer population in this study were most significantly associated with ADFI. Many of these markers were also associated with the related traits of ADG and/or RFI (P, nominal ≤0.05). Even though ADG and RFI associations were only nominally significant, their effects were in the expected direction (alleles with higher ADFI effects had higher ADG and RFI effects). In general, alleles that are associated with higher feed intakes, when also nominally significant for other traits, produced greater HCW and greater fat deposition. However, ribeye area and tenderness were not affected suggesting that the ribeye, and possibly other lean muscles, were not affected by the increased fat deposition.

One marker, 77244_529, was nominally associated with ADFI, ADG, and RFI in our discovery population. An animal with the G allele at this marker would be predicted to have a reduced feed consumption of 27.9 kg over a 140-day-feeding period, which would be a significant cost savings at the feedlot. However, feed intake is a complex trait and since multiple genetic and environmental factors contribute to an animal’s consumption of feed, these effects are not likely to be realized to this extent in different populations with this marker. Moreover, this marker was not significant in our validation population, suggesting a population specific association. Our genetic marker data indicated that the variation in the chemerin gene may be responsible for some of the observed ADFI variation in our discovery population; however, the lack of validation of these markers suggested that they may not be particularly robust across breeds and populations.

Additional studies within this region may be necessary to identify markers that are more useful across cattle populations. There is recent evidence that the gene expression of replication inhibitor 1 (Repin1) may be involved in metabolic disorder in rats (Bahr et al., 2011). A strain of rats (BB.4W) that develop obesity, dyslipidemia, impaired glucose tolerance, hyperinsulinemia, and hyperleptinemia displayed lower relative transcript abundance of Repin1 in adipose tissue. In cattle, REPIN1 is located within close proximity of the chemerin gene suggesting that studies to evaluate whether REPIN1 expression plays a role in cattle feed intake are warranted.

We performed SNP association analysis on heifers (n = 114) related to the discovery steer population and detected a few markers that were approaching significance with ADFI and RFI (P ≤ 0.1; data not shown). This analysis was likely under-powered due to the limited number of heifers. However, these associations, the associations from the related discovery population of steers, and the half to partial sibling relationships between these two groups of animals provided support for the use of the heifer adipose tissue as an appropriate source to evaluate chemerin gene expression.

We found that chemerin gene expression in the adipose tissue of heifers was correlated to their BCS and yearling weight. A previous study has shown a relationship between chemerin expression, adipogenesis and leptin (Goralski et al., 2007). RNA transcripts for chemerin and its receptor were found to be highly expressed in mouse white adipose tissue, which is responsible for energy storage (Goralski et al., 2007). This study also showed that chemerin was expressed at higher levels in differentiated adipocytes and chemerin, and its receptor, appeared to be necessary for adipocyte differentiation. In a post-differentiation chemerin knockdown experiment, performed in an adipocyte cell culture model, leptin gene expression was reduced (Goralski et al., 2007). These data provide evidence for a potential role of chemerin in cattle feed intake, as its effects on circulating leptin would alter appetite. In addition, a relationship between adipogenesis and chemerin expression may account for a portion of the variation in cattle BCS. Both adipogenesis and an effect on the leptin appetite pathway could affect an animal’s feed intake phenotype and its overall level of body fat.

In summary, we have detected several polymorphisms within a region on bovine chromosome 4, which includes the chemerin gene, that were significantly associated with feed intake in a discovery population of cattle. In general, the alleles that were associated with higher feed intakes were associated with higher HCW, AFT, and marbling, but no association with REA and tenderness was detected; thus, fat accretion may be responsible for the increase in HCW. However, we were not able to validate these associations in another population of cattle. Chemerin gene expression in the adipose tissue of heifers was greater in animals with greater BCS and yearling weights supporting data from human and mouse studies that indicate a relationship between chemerin and fat deposition.

Conflict of Interest Statement

Mention of trade name proprietary product or specified equipment does not constitute a guarantee or warranty by the USDA and does not imply approval to the exclusion of other products that may be suitable. USDA is an equal opportunity provider and employer.

Acknowledgments

The authors appreciate the excellent technical assistance provided by Linda Flathman and Kris Simmerman. We also thank Donna Griess for manuscript preparation, and the USMARC cattle operations employees for animal care and management.

Footnotes

  1. ^Mention of trade names or commercial products in this publication is solely for the purpose of providing specific information and does not imply recommendation or endorsement by the U.S. Department of Agriculture.
  2. ^USDA is an equal opportunity provider and employer.
  3. ^http://frodo.wi.mit.edu
  4. ^http://www.phrap.org
  5. ^http://www.broad.mit.edu/mpg/haploview/index.php

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Keywords: average daily feed intake, beef cattle, BTA4, chemerin, feed intake, RARRES2

Citation: Lindholm-Perry AK, Kuehn LA, Rempel LA, Smith TPL, Cushman RA, McDaneld TG, Wheeler TL, Shackelford SD, King DA and Freetly HC (2012) Evaluation of bovine chemerin (RARRES2) gene variation on beef cattle production traits. Front. Gene. 3:39. doi: 10.3389/fgene.2012.00039

Received: 15 November 2011; Accepted: 29 February 2012;
Published online: 29 March 2012.

Edited by:

Peter Dovc, University of Ljubljana, Slovenia

Reviewed by:

Georgia Hadjipavlou, Agricutlural Research Institute, Cyprus
Nora Lía Padola, Universidad Nacional del Centro de la Provincia de Buenos Aires, Argentina

Copyright: © 2012 Lindholm-Perry, Kuehn, Rempel, Smith, Cushman, McDaneld, Wheeler, Shackelford, King and Freetly. This is an open-access article distributed under the terms of the Creative Commons Attribution Non Commercial License, which permits non-commercial use, distribution, and reproduction in other forums, provided the original authors and source are credited.

*Correspondence: Amanda K. Lindholm-Perry, U.S. Meat Animal Research Center, Agricultural Research Service, United States Department of Agriculture, P. O. Box 166, State Spur 18D, Clay Center, NE 68933-0166, USA. e-mail: amanda.lindholm@ars.usda.gov

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