Immunocytochemical staining of knock-down HeLa clones. Long-term silenced clones were propagated in culture and analyzed (one representative field is shown for each clone; Magnification ×100).

Functional analysis of NHEJ-deficient HeLa cells. Protein contents were analyzed (A) by immunocytochemical staining (DNA PKcs^KD cells at day 176 after UVC or γ ray irradiation) or (B) by western blotting. 1: Control (pBD650); 2: DNA PKcs ^KD cl.1 (pBD743; day 94); 3: XRCC4^KD cl.9 (pBD694; day 94). (C) NHEJ activities were measured using an in vitro NHEJ assay. Agarose gel separation of NHEJ products was followed by Southern blotting. Reaction products are marked on the right side: M: linear multimers (inter-molecular joining); OC: open circles (intra-molecular joining); LIN: input linear substrate; CC: covalently closed circles (intra-molecular joining). 1: Control (pBD650); 2: XRCC4^KD cl.9 (pBD694; day 75). 3: DNA PKcs^KD cl.1 (pBD743; day 75); 4: Control (pBD650); 5: KIN17^KD cl.6 (pBD674; day 81). 6: KIN17^KD cl.12 (pBD674; day 81).

(A) Cell cycle progression of stable knock-down HeLa clones after UVC (10 J/m²), γ rays (6 Gy) or etoposide treatment (VP16; 25 μM for 1.5 h): GG-NER and TC-NER pathways. Exponentially growing cells were treated and 24 h later adherent cells were collected, washed and fixed in 75% ethanol at 4°C for at least 24 h. Cells were stained with propidium iodide (4 μg/ml) in the presence of RNase (10 μg/ml) for at least 30 min. Stained cells were analyzed on a FACScalibur (Becton Dickinson) using CellQuest software. Here, ∼10 000 cells gated as single cells using FL2A/FL2W scatter were analyzed. Each clone was analyzed at least three times. Long-term HeLa clones: Control (BD650, day115), XPC^KD (BD634/21; day 333), hHR23A^KD (BD805/7; day 158), hHR23B^KD (BD804/9; day 191), XPA^KD (BD695/6; day 422). Arrows indicate a striking point highlighting intolerance to DNA damage. (B) NHEJ and HR pathways. Long-term HeLa clones: DNAPKcs^KD (BD743/1; day 321), XRCC4^KD (BD694/9; day 235), LigIV^KD (BD940/3; day 103), LigIII^KD (BD941/11; day 82), Rad51^KD (BD864/2; day 107), Rad54^KD (BD912/5; day 148). (C) Signaling pathways Long-term HeLa clones: MRE11^KD (BD930/32; day 61), Rad50^KD (BD872/1; day 158), NBS1^KD (BD932/11; day 108), ATM^KD (BD935/12; day 111), ATR^KD (BD962/9; day 56).

Protein analysis of long-term LigIII^KD, LigIV^KD, XRCC4^KD and CSB^KD clones.

Short- and long-term gene silencing for MRN components. (A and B) 45, 69 and 76 days after transfection, Rad50^KD HeLa clones were analyzed by immunocytochemical staining (magnification ×315) or western blot. 1: Control (pBD650; day 189); 2: XPC^KD cl. 21 (pBD634; day 376); 3: XPA^KD clone 6 (pBD695; day 436); 4: XRCC4^KD clone 9 (pBD694; day 107); 5: Control (pBD650; day 31); 6: Rad50^KD clone 1 (pBD872; day 76); 7: Rad50^KD clone 1 (day 45); 8: Rad50^KD clone 2 (day 45); 9: Rad50^KD clone 3 (day 45); 10: Rad50^KD clone 4 (day 45); 11: Rad50^KD clone 5 (day 45). (C) Transient gene silencing: 6 days after transfection, MRE11^KD (two pEBVsiRNA plasmids), Rad50^KD (one plasmid) and NBS1^KD (two plasmids) cell populations were analyzed by western blot. 1: Control (pBD650; day 6); 2: MRE11^KD (pBD930; day 6); 3: MRE11^KD (pBD931; day 6); 4: NBS1^KD (pBD932; day 6); 5: NBS1^KD (pBD934; day 6); 6: ATM^KD (pBD935; day 6); 7: ATM^KD (pBD936; day 6); 8: ATM^KD (pBD937; day 6); 9: PARG^KD (pBD812; day 6); 10: Rad50^KD (pBD872; day 6); 11: Control (pBD650; day 6); 12: Rad50^KD (day 120). (D) Long-term gene silencing: Clones were picked up from cell populations described in the panel ‘C’ and propagated for several months in culture. 1: Control (pBD650; day 238); 2: MRE11^KD cell population (pBD930; day 33); 3: MRE11^KD clone 32 (pBD930; day 132); 4: Rad50^KD clone 1 (pBD872; day 149); 5: NBS1^KD clone 11 (pBD932; day 172); 6: DNA PKcs^KD clone 1 (pBD743; day 391); 7: Ligase III^KD clone 11 (pBD941; day 180).

Clonogenic cell survival assays after UVC (4 J/m²), γ rays (1 Gy) or etoposide treatment (VP16; 1 μM for 1.5 h). Established long-term clones were seeded at 500 cells per 6-cm diameter-dish 24 h before treatment. Here, ∼14 days later, cells were fixed and stained. Each point represents the mean of two independent experiments; each experiment represents three culture dishes per point. SD are indicated. Age of cells at the time of the last clonogenic cell survival assay: Control (pBD650; day 238); XPC^KD cell cl.21(day 456); hHR23A^KD cl.7 (day 236); hHR23B^KD cl.9 (day 272); DNA PKcs^KD cl. 1 (day 365); XRCC4^KD cl.9 (day 205); Ligase IV^KD cl.3 (day 176); Ligase III^KD cl.11 (day 178); Rad51^KD cl.2 (day 193); Rad54^KD cl.5 (day 322); MRE11^KD cl.32 (day 177); Rad50^KD cl.1 (day 175); NBS1^KD cl.11 (day 176); ATM^KD cl.12 (day 302); ATR^KD cl.9 (day 196); Ogg1^KD cl.27 (day 232). Arrows indicate a striking point highlighting intolerance to DNA damage.