(A) Scheme depicting shRNA (luc29) or siRNA (siluc) against Firefly luciferase, plus competitors (H25 shRNA and sigfp siRNA). (B) New Huh-7 cell lines stably overexpressing human Ago-2 (8 representative examples; all studies were performed in clone 1 [arrow] and validated in clone 2). Arrow indicates the best-expressing cell line, in which all studies were performed. (C) Huh-7 cells were cotransfected with: (a) Firefly (target) and Renilla (normalization) luciferase, (b) shRNA expression plasmid (encoding H25 or luc29 shRNA, or only U6 promoter), (c) plasmids encoding Ago-1 or -2 (or CMV promoter as control), (d) anti-gfp competitor siRNA (sigfp), and (e) anti-luciferase siRNA (siluc). Ago-2 overexpression enhanced basal luc siRNA activity and diminished competition with gfp siRNA or H25 shRNA (green arrows). Ago-2 likewise enhanced luciferase knockdown when cotransfected with luc29 shRNA (plus or minus luc siRNA; orange arrows). Ago-1 overexpression had no significant effect on the siRNA, but also reduced si/shRNA competition (red arrow), perhaps by sequestering the shRNA and thus freeing Ago-2/RISC for the siRNA. P < 0.05, all Ago-2 bars labeled with green/orange arrows versus controls. (D) Confirmation of the Ago-2 effects in a different cell line. (E) Validation in stable Ago-2 Huh-7 cells (see B), transfected with Firefly/Renilla, various RNAi triggers (siRNA, esiRNA, or shRNA, as indicated) against Firefly, and Ago expression plasmids (or a control). Basal siRNA, esiRNA (enzymatically created siRNA), and shRNA activities were all elevated (red) compared with parental Huh-7 (blue), confirming that Ago-2 restricts all classes of perfect RNAi duplexes. (F) Repeat of the transfections from C in stable Ago-2 cells. Competition between 2 siRNAs, or between luc siRNA and H25 shRNA, was greatly diminished compared with that in the parental cells (C). (G) Transfection of all perfect RNAi duplexes into Ago-2–deficient MEFs confirmed their strict Ago-2 dependence.