Figure 3.
MyD88–/– and TLR2–/–BMMϕs show impaired MAPK activation and TNF-α production upon mycobacterial infection. BMMϕs from WT and TLR2–/– mice (A-B) and MyD88–/– mice (C-D) were infected with M smegmatis or M avium 724 and screened for MAPK activation at 1 hour and 9 hours and TNF-α production at 24 hours. (A,C) MAPK activation was detected by preparing cell lysates after 1-hour and 9-hour infections and probed for activated ERK1/2 and p38 using phospho-specific Abs as described in “Materials and methods.” Total ERK1/2 and p38 blots were run to show equal protein loading. (B,D) BMMϕs from WT and KO mice were infected with complement opsonized or nonopsonized mycobacteria; 24 hours later, culture supernates were removed and analyzed by ELISA for TNF-α. Values are expressed as means + SD. Data are representative of 3 separate experiments. Sm and Smeg indicate M smegmatis; Av and Avium, M avium; and RC, noninfected BMMϕs.

MyD88–/– and TLR2–/–BMMϕs show impaired MAPK activation and TNF-α production upon mycobacterial infection. BMMϕs from WT and TLR2–/– mice (A-B) and MyD88–/– mice (C-D) were infected with M smegmatis or M avium 724 and screened for MAPK activation at 1 hour and 9 hours and TNF-α production at 24 hours. (A,C) MAPK activation was detected by preparing cell lysates after 1-hour and 9-hour infections and probed for activated ERK1/2 and p38 using phospho-specific Abs as described in “Materials and methods.” Total ERK1/2 and p38 blots were run to show equal protein loading. (B,D) BMMϕs from WT and KO mice were infected with complement opsonized or nonopsonized mycobacteria; 24 hours later, culture supernates were removed and analyzed by ELISA for TNF-α. Values are expressed as means + SD. Data are representative of 3 separate experiments. Sm and Smeg indicate M smegmatis; Av and Avium, M avium; and RC, noninfected BMMϕs.

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