To analyze SCAs-formation, mFISH analysis and classical cytogenetic analysis were employed. Briefly, 2.5 × 106 cells transfected with pCMV-3xNLS-ISceI plasmid were split in three dishes and plated for 24, 30 and 48 h, respectively. To accumulate cells at metaphase, colcemid (Biochrom AG) was added for 2–3 h at a concentration of 0.1 μg/ml. Metaphase spreads were prepared using standard procedures. mFISH was performed using 12XCHamster Multicolor FISH Probe for Chinese Hamster Chromosomes (MetaSystems Probes) according to manufacturer’s protocol. An automated imaging system (MetaSystems) was used to obtain high quality images of metaphase chromosomes, as previously described (Soni et al., 2019 (link)). For analysis, at least 100 metaphases were scored in each of three independent experiments. The number of the SCAs formed in the non-transfected clones is subtracted from the SCAs number in cells transfected with I-SceI expressing plasmid.
Classical cytogenetic methods were also employed, as previously described (Schipler et al., 2016 (link)). High quality images of metaphase chromosomes were captured using Zeiss AxioScan.Z1 imaging platform at a magnification of ×40 dry objective. Images were analyzed using the integrated ZEN software. For analysis, at least 100 metaphases were scored in each of three independent experiments.
Classical cytogenetic methods were also employed, as previously described (Schipler et al., 2016 (link)). High quality images of metaphase chromosomes were captured using Zeiss AxioScan.Z1 imaging platform at a magnification of ×40 dry objective. Images were analyzed using the integrated ZEN software. For analysis, at least 100 metaphases were scored in each of three independent experiments.
Free full text: Click here
