Phosphate-buffered saline (PBS), pH 7.4, to block endogenous peroxidase. Antigen unmasking was

August 17, 2017

Phosphate-buffered saline (PBS), pH 7.4, to block endogenous peroxidase. Antigen unmasking was performed with pepsin (15 min, Sigma, St Louis, USA). To minimize nonspecific binding, sections were incubated with serum blocking solution (HistostainH Bulk Kit, Invitrogen Corporation, Carlsbad, California) and subsequently incubated overnight with primary antibodies in a moist HIF-2��-IN-1 cost chamber at 4uC. Information on primary antibodies is provided in Table 1. On the second day, immunohistochemistry was performed with standard procedures using HistostainH Bulk Kit (Invitrogen Corporation, Carlsbad, California). The immunostaining reaction product was developed using 0.1 g diaminobenzidine (DAB) (3,39,4,49 etraminobiphenyl, Sigma, St Louis, USA) in 200 ml of PBS, plus 40 ml hydrogen peroxide. After immunoreactions,Care and handling of the BTZ043 animals and the storage of the samplesAll animals used had an attending veterinarian available, and health status was monitored at least once daily. Clinical specificLPA1 in Prostate Dysplastic LesionsTable 1. Primary antibodies used for immunohistochemistry.Antigen LPA1(EDG2) UBIQUITIN Von Willebrand Factor (Factor VIII) PCNA MCM7 Bcl2 pConcentration 1:100 1:200 Ready to use 1:100 1:50 1:100 1:Supplier Novus Biologicals, Litttleton. USA DAKO Carpinteria, California. USA DAKO Carpinteria, California. USA Biomeda, Foster City, CA Oncogene. Cambridge. MA. USA DAKO Carpinteria, California. USA Cell Signaling, Beverly, MASource PolyclonalMonoclonaldoi:10.1371/journal.pone.0057742.tsections were counterstained with acetic carmine, Harris hematoxylin, or methyl green, dehydrated in ethanol and mounted in a synthetic resin (Depex, Serva, Heidelberg, Germany). The specificity of the immunohistochemical procedures was checked by incubation of sections with nonimmune serum instead of the primary antibody.Quantitative evaluation of Bcl-2 immunostainingTo quantify the immunoreactivity of Bcl-2 protein, its volume fraction (VF) was measured and expressed as percentage of immunostained epithelium. Estimation of the VF was performed using the ImageJ v1.45 program. The selected fields were photographed, thresholded, and binarized, and the percentage of epithelial area was automatically measured by the program to obtain the VF [7]. The VF of Bcl-2 immunoreactivity was estimated in ventral prostates from the control and experimental animals to ascertain if treatment changes the total amount of Bcl-2 immunostaining in the epithelium. This estimation was measured in each selected section from control rats, nondysplastic acini of Cd-treated rats, and dysplastic acini of Cd-treated rats.DNA fragmentation detectionTo detect the apoptotic fragmentation of DNA, a TUNEL (TdT-mediated dUTP-biotin nick end labeling) technique (Boehringer Mannheim) was used [6,28]. This method involves the insertion of labeled nucleotides into broken ends of DNA strands. A brief description of the method follows: sections were deparaffinized 12926553 and rehydrated and then incubated with proteinase K (10 ml/ml in TRIS/EDTA pH 8) for 30 min at 37uC for digestion of nuclear proteins. Endogenous peroxidase was inactivated with 0.3 hydrogen peroxide in distillate water during 30 min. The sections were incubated for 1 hr at 37uC in the TdT (terminal deoxynucleotide transferase) mixture with addition of labeled nucleotides (2:1), and after that, they were incubated in converter POD during 30 min at 37uC. The reaction was detected using 0.1 g DAB in PBS (200 ml), plus 40 ml hy.Phosphate-buffered saline (PBS), pH 7.4, to block endogenous peroxidase. Antigen unmasking was performed with pepsin (15 min, Sigma, St Louis, USA). To minimize nonspecific binding, sections were incubated with serum blocking solution (HistostainH Bulk Kit, Invitrogen Corporation, Carlsbad, California) and subsequently incubated overnight with primary antibodies in a moist chamber at 4uC. Information on primary antibodies is provided in Table 1. On the second day, immunohistochemistry was performed with standard procedures using HistostainH Bulk Kit (Invitrogen Corporation, Carlsbad, California). The immunostaining reaction product was developed using 0.1 g diaminobenzidine (DAB) (3,39,4,49 etraminobiphenyl, Sigma, St Louis, USA) in 200 ml of PBS, plus 40 ml hydrogen peroxide. After immunoreactions,Care and handling of the animals and the storage of the samplesAll animals used had an attending veterinarian available, and health status was monitored at least once daily. Clinical specificLPA1 in Prostate Dysplastic LesionsTable 1. Primary antibodies used for immunohistochemistry.Antigen LPA1(EDG2) UBIQUITIN Von Willebrand Factor (Factor VIII) PCNA MCM7 Bcl2 pConcentration 1:100 1:200 Ready to use 1:100 1:50 1:100 1:Supplier Novus Biologicals, Litttleton. USA DAKO Carpinteria, California. USA DAKO Carpinteria, California. USA Biomeda, Foster City, CA Oncogene. Cambridge. MA. USA DAKO Carpinteria, California. USA Cell Signaling, Beverly, MASource PolyclonalMonoclonaldoi:10.1371/journal.pone.0057742.tsections were counterstained with acetic carmine, Harris hematoxylin, or methyl green, dehydrated in ethanol and mounted in a synthetic resin (Depex, Serva, Heidelberg, Germany). The specificity of the immunohistochemical procedures was checked by incubation of sections with nonimmune serum instead of the primary antibody.Quantitative evaluation of Bcl-2 immunostainingTo quantify the immunoreactivity of Bcl-2 protein, its volume fraction (VF) was measured and expressed as percentage of immunostained epithelium. Estimation of the VF was performed using the ImageJ v1.45 program. The selected fields were photographed, thresholded, and binarized, and the percentage of epithelial area was automatically measured by the program to obtain the VF [7]. The VF of Bcl-2 immunoreactivity was estimated in ventral prostates from the control and experimental animals to ascertain if treatment changes the total amount of Bcl-2 immunostaining in the epithelium. This estimation was measured in each selected section from control rats, nondysplastic acini of Cd-treated rats, and dysplastic acini of Cd-treated rats.DNA fragmentation detectionTo detect the apoptotic fragmentation of DNA, a TUNEL (TdT-mediated dUTP-biotin nick end labeling) technique (Boehringer Mannheim) was used [6,28]. This method involves the insertion of labeled nucleotides into broken ends of DNA strands. A brief description of the method follows: sections were deparaffinized 12926553 and rehydrated and then incubated with proteinase K (10 ml/ml in TRIS/EDTA pH 8) for 30 min at 37uC for digestion of nuclear proteins. Endogenous peroxidase was inactivated with 0.3 hydrogen peroxide in distillate water during 30 min. The sections were incubated for 1 hr at 37uC in the TdT (terminal deoxynucleotide transferase) mixture with addition of labeled nucleotides (2:1), and after that, they were incubated in converter POD during 30 min at 37uC. The reaction was detected using 0.1 g DAB in PBS (200 ml), plus 40 ml hy.