Our findings
may reduce the serious lack of information and controversial studies concerning the toxicological effects of engineering gold nanoparticles. Chemicals were obtained from Sigma–Aldrich (USA). Glutamine, penicillin/streptomycin, fetal bovine serum, cell culture media were purchased from Cultilab (Brazil). Doxorubicin (DXR) was used in commercial formula: Adriblastin1 RD (CAS: 25316-40-9, Pharmacia and Upjohn, Milan, Italy). AuNps were chemically SB203580 in vivo synthesized in the presence of PAMAM or sodium citrate, leading to the formation of AuNps with diameters ranging from 7 to 20 nm, bearing positive and negative charges, respectively. Details on the synthesis of the Nps-PAMAM can be found elsewhere (Crespilho et al., 2007). Briefly, 2 mL of PAMAM G4 (0.07 mmol L−1) were added to 2 mL of HAuCl4 solution (1 mmol L−1) and Epacadostat purchase 2 mL of formic acid 10% (v/v). This solution was mixed and shaked during 4 h. The color changed from yellow to red, indicating
the zerovalent Au complex was formed after 4 h. The AuNps-citrate were obtained by citrate reduction of gold salts, as previously described (Grabar et al., 1995). Briefly, 1.0 mL of 1% sodium citrate was added to 14 mL of boiling solution 0.5 mmol L−1 HAuCl4 with vigorous stirring. The final solution color changes
to red–violet rapidly. The nanoparticle formation was monitored by UV–vis spectrophotometry (Hitachi U-2001 Spectrophotometer; San Jose, CA, USA). AuNPs morphology and particle size distribution were estimated by transmission electron microscopy (TEM, Model CM200; Philips, the Netherlands) by measuring at least 100 particles in TEM images using the program Image J (Java-Sun Microsystems). Typical AuNPs TEM images used in this study are shown in Fig. 1. The Zeta potential and the hydrodynamic diameter were measured (Malvern Zetasizer) before and after AuNp dilution into cell culture medium with serum (10% fetal bovine serum-FBS) Idoxuridine (Table 1). The citrate or PAMAM excess was removed upon successive centrifugation and rinsing steps using phosphate buffer saline 0.05 M (PBS) solution. After each centrifugation, the AuNps were resuspended in 0.05 M PBS at pH 7.0 following the discard of the supernatant. The process was repeated three times to eliminate the free citrate or PAMAM molecules. The AuNps were then diluted in cell culture medium. Finally, the AuNps were sonicated for 30 min before using. Whole peripheral blood was collected from women and men adult healthy volunteers, no tobacco users, no pregnant women.