Hoechst 35,528 (Sigma, St Louis, MA, USA), a nuclear dye, was app

Hoechst 35,528 (Sigma, St Louis, MA, USA), a nuclear dye, was applied to reveal tissue architecture. Tissue autofluorescence in sections from adult Copanlisib mouse and primate brains was quenched with Sudan Black B (Schnell et al., 1999). Sections were inspected and representative images of immunoreactivity were acquired on a Zeiss 710LSM confocal laser-scanning microscope (Zeiss, Jena, Germany) equipped to separate emission signals through spectral detection and

unmixing. Emission spectra for each dye was limited as follows: Hoechst (420–485 nm), Cy2 (505–530 nm), Cy3 (560–610 nm) and Cy5 (640-720 nm). Image surveys were generated using the tile scan function with optical zoom varied from 0.6× to 1.5× at 10× primary magnification (objective: EC Plan-Neofluar 10×/0.30). Co-localization was defined as immunosignals being Torin 1 solubility dmso preset without physical signal separation in ≤ 1.0-μm optical slices at 40× (Plan-Neofluar 40×/1.30) or 63× (Plan-Apochromat 63×/1.40) primary magnification (Mulder et al., 2009b). Images were processed using the ZEN2009 software (Zeiss). Multi-panel

figures were assembled in CorelDraw X3 (Corel Corp., Ottawa, ON, Canada). The diameter of scgn+ neurons was measured after capturing images of scgn+ cell assemblies in pallidal and EA territories at 40× primary magnification. The somatic diameter of individual neurons was measured on the premise that scgn is a cytosolic protein (Attems 3-mercaptopyruvate sulfurtransferase et al., 2007) and is homogenously distributed throughout the neuronal perikarya. Only neurons with smooth surfaces and processes were included in our analysis to avoid bias due to partial profiles of cell fragments. Serial coronal sections (sampling interval, 140 μm) spanning the entire forebrain from an E15 mouse were double-labelled to reveal scgn+ neurons and cell nuclei (Hoechst 35,528). Single x-y plane images were acquired (Zeiss 710LSM), and 3-D-reconstructed using the BioVis3D software (BioVis3D, Montevideo, Uruguay). Data are expressed as means ± SEM and analyzed using Student’s t-test (spss

v.16.0, SPSS Inc., Chicago, IL, USA). A P-value of < 0.05 was considered statistically significant. Human fetal specimens at mid-gestation (21–22 weeks of gestation; n = 3) were obtained from saline-induced abortions (Wang et al., 2004; Hurd et al., 2005). Protocols were approved by the local institutional review board (Institutional Review Boards of Kings County Hospital Center and Downstate Medical Center, State University of New York) as part of a large-scale study to evaluate the molecular effects of prenatal drug exposure on human neurodevelopment (Hurd et al., 2005). Specimens were fixed in 1% PFA and frozen at −80°C. Coronal cryosections (20 μm) spanning corticolimbic areas including the amygdaloid complex were cut. In situ hybridization was conducted as described (Wang et al.

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