For negative staining EM grid preparation, samples (5 µL at a concentration of ~0.035 mg/mL) were applied onto glow-discharged copper grids supported by a continuous thin layer of carbon film for 60 s before being negatively stained by 2% (w/v) uranyl formate solution at room temperature. The grids were prepared in the Ar/O2 mixture for 15 s using a Gatan 950 Solarus plasma cleaning system with a power of 35 W. The negatively stained grids were loaded onto a Thermo Fisher Scientific Talos L120C microscope equipped with a Ceta CCD camera and operated at 120 kV at a nominal magnification of 92,000×, corresponding to a pixel size of 1.58 Å on the specimen.
For cryo-EM grid preparation, samples (4 μL at a concentration of ~1.5 mg/mL) were applied to freshly glow-discharged Quantifoil R1.2/1.3 holey gold grids. After incubation for 5 s at 4 °C and 100% humidity, the grids were blotted for 8.5 s with force 13 in a Thermo Fisher Scientific Vitrobot Mark IV and plunge-frozen in liquid ethane at liquid nitrogen temperature. The grids were prepared in the H2/O2 mixture for 20 s using a Gatan 950 Solarus plasma cleaning system with a power of 5 W. The ø 55/20 mm blotting paper (TED PELLA) was used for plunge freezing.
For cryo-EM grid preparation, samples (4 μL at a concentration of ~1.5 mg/mL) were applied to freshly glow-discharged Quantifoil R1.2/1.3 holey gold grids. After incubation for 5 s at 4 °C and 100% humidity, the grids were blotted for 8.5 s with force 13 in a Thermo Fisher Scientific Vitrobot Mark IV and plunge-frozen in liquid ethane at liquid nitrogen temperature. The grids were prepared in the H2/O2 mixture for 20 s using a Gatan 950 Solarus plasma cleaning system with a power of 5 W. The ø 55/20 mm blotting paper (TED PELLA) was used for plunge freezing.