Extended Data Fig. 2 |. Immunoblot characterization of purified VZV capsids.

VZV capsids (c) were purified from the infected ARPE-19 cells at 3 dpi and were analyzed by western blot using antibodies against the indicated viral proteins. Lysates of uninfected (−) and VZV-infected (+) cells were used as negative and positive controls, respectively. Molecular mass markers in kilodaltons (kDa) are shown on the left. Experiments were performed two times independently with similar results. pORF43 and pORF34 of VZV are homologs of pUL17 and pUL25 of HSV-1, respectively, and represent two putative components (c1 and c2) of VZV CATC.