Ment and Accreditation of Laboratory Animal Care International Standards and with

September 18, 2017

Ment and Accreditation of Laboratory Pluripotin animal Care International Standards and with the recommendations in the Guide for the Care and Use of Laboratory Animals of the National Institutes of Health. The Institutional Animal Use and Care Committee of the University of California, Davis, approved these experiments (Protocol # 15835). When immobilization was necessary, the animals were injected intramuscularly with 10 mg/kg of Ketamine HCl (Parke-Davis, Morris Plains N.J.). All efforts were made to minimize suffering. Details of animal welfare and steps taken to ameliorate suffering were in accordance with the recommendations of the Weatherall report, “The use of non-human primates in research”. Animals were housed in an air-conditioned facility with an ambient temperature of 21?5uC, a relative humidity of 40 ?0 and a 12 h light/ dark cycle. Animals were individually housed in suspendedAmplification of Cytokine, and Interferon-stimulated Genes by Reverse Transcriptase Real-time PCRTotal RNA was isolated from CVS samples using Trizol (Invitrogen, Grand Island, NY) according to the manufacturer’s protocol. All samples were DNase-treated with DNA-free (Ambion) for 1 hr. at 37uC. cDNA was prepared using random primers and Superscript II (both from Invitrogen). Real-Time PCR was performed using the ABI 7900 Real-Time PCR System (Applied Biosystems, Foster City, CA) as previously described [23?Cervicovaginal Inflammation in Rhesus MacaquesFigure 2. Comparison of relative concentration of for pro-inflammatory cytokine/chemokine mRNAs in vaginal secretions of RM in samples are similar. A) IL-6, B) TNF, C) MIP-1a, D) MIP-1b, E) IFNa, F) MIG. Time 1 indicates the CVS samples were BI 78D3 site collected in March 2011. Time 2 indicates that the CVS samples were collected in November 2011. All vaginal secretions were collected between menstrual cycle days 10?0. doi:10.1371/journal.pone.0052992.g25]. Briefly, samples were tested in duplicate and the PCR for the housekeeping gene GAPDH and the target gene were run in parallel on the same plate. The PCR reaction was carried out on a 96 well Optical Plate (Applied Biosystems) in a 25 ml reaction volume containing 5 ml cDNA +20 ml Mastermix (Applied Biosystems). All PCR reactions were run on using the default amplification program: 2 min. at 50uC, 10 min. at 95uC, followed by 45 cycles of 15 s at 95uC and 1 min. at 60uC. Results were analyzed with the SDS 7900 system software, version 2.1 (AppliedBiosystems). The mRNA expression levels were calculated from normalized delta Ct (DCt) values. Ct values correspond to the cycle number at which the fluorescence due to enrichment of the PCR product reaches significant levels above the background fluorescence (threshold). In this analysis, the Ct value for the housekeeping gene (GAPDH) is subtracted from the Ct value of the target gene. For vaginal lavage samples, the target cytokine mRNA levels in a sample are expressed as the fold increase relative to the GAPDH mRNA levels in the same sample. Also note thatCervicovaginal Inflammation in Rhesus MacaquesFigure 3. Network of 1527786 statistical correlations between mRNA levels of immune mediators. After unbiased analysis of potential associations between the levels of every mRNA levels measured using a Spearman’s correlation function there was a limited network of strong (.0.7) correlations between mRNA levels of A) 3 cytokine/chemokines at Time point 1; B) 3 cytokines/chemokines; and 2 Interferon-stimulated genes at Time point 2. C) ne.Ment and Accreditation of Laboratory Animal Care International Standards and with the recommendations in the Guide for the Care and Use of Laboratory Animals of the National Institutes of Health. The Institutional Animal Use and Care Committee of the University of California, Davis, approved these experiments (Protocol # 15835). When immobilization was necessary, the animals were injected intramuscularly with 10 mg/kg of Ketamine HCl (Parke-Davis, Morris Plains N.J.). All efforts were made to minimize suffering. Details of animal welfare and steps taken to ameliorate suffering were in accordance with the recommendations of the Weatherall report, “The use of non-human primates in research”. Animals were housed in an air-conditioned facility with an ambient temperature of 21?5uC, a relative humidity of 40 ?0 and a 12 h light/ dark cycle. Animals were individually housed in suspendedAmplification of Cytokine, and Interferon-stimulated Genes by Reverse Transcriptase Real-time PCRTotal RNA was isolated from CVS samples using Trizol (Invitrogen, Grand Island, NY) according to the manufacturer’s protocol. All samples were DNase-treated with DNA-free (Ambion) for 1 hr. at 37uC. cDNA was prepared using random primers and Superscript II (both from Invitrogen). Real-Time PCR was performed using the ABI 7900 Real-Time PCR System (Applied Biosystems, Foster City, CA) as previously described [23?Cervicovaginal Inflammation in Rhesus MacaquesFigure 2. Comparison of relative concentration of for pro-inflammatory cytokine/chemokine mRNAs in vaginal secretions of RM in samples are similar. A) IL-6, B) TNF, C) MIP-1a, D) MIP-1b, E) IFNa, F) MIG. Time 1 indicates the CVS samples were collected in March 2011. Time 2 indicates that the CVS samples were collected in November 2011. All vaginal secretions were collected between menstrual cycle days 10?0. doi:10.1371/journal.pone.0052992.g25]. Briefly, samples were tested in duplicate and the PCR for the housekeeping gene GAPDH and the target gene were run in parallel on the same plate. The PCR reaction was carried out on a 96 well Optical Plate (Applied Biosystems) in a 25 ml reaction volume containing 5 ml cDNA +20 ml Mastermix (Applied Biosystems). All PCR reactions were run on using the default amplification program: 2 min. at 50uC, 10 min. at 95uC, followed by 45 cycles of 15 s at 95uC and 1 min. at 60uC. Results were analyzed with the SDS 7900 system software, version 2.1 (AppliedBiosystems). The mRNA expression levels were calculated from normalized delta Ct (DCt) values. Ct values correspond to the cycle number at which the fluorescence due to enrichment of the PCR product reaches significant levels above the background fluorescence (threshold). In this analysis, the Ct value for the housekeeping gene (GAPDH) is subtracted from the Ct value of the target gene. For vaginal lavage samples, the target cytokine mRNA levels in a sample are expressed as the fold increase relative to the GAPDH mRNA levels in the same sample. Also note thatCervicovaginal Inflammation in Rhesus MacaquesFigure 3. Network of 1527786 statistical correlations between mRNA levels of immune mediators. After unbiased analysis of potential associations between the levels of every mRNA levels measured using a Spearman’s correlation function there was a limited network of strong (.0.7) correlations between mRNA levels of A) 3 cytokine/chemokines at Time point 1; B) 3 cytokines/chemokines; and 2 Interferon-stimulated genes at Time point 2. C) ne.