EcMinC fused with the N-terminal chloroplast transit peptide from

EcMinC fused with the N-terminal chloroplast transit peptide from Rubisco small subunit and a C-terminal GFP was transiently expressed in I-BET-762 mouse Arabidopsis protoplasts. Interestingly, EcMinC-GFP was localized to puncta in chloroplasts AMN-107 purchase (Figure 4G, H and 4I), a pattern similar to that of AtMinD-GFP in chloroplasts [20, 24]. This probably is because the endogenous AtMinD has a punctate localization pattern and it can interact with EcMinC-GFP. It has been shown that overexpression of chloroplast-targeted EcMinC

in plants inhibits the division of chloroplasts [25]. In E. coli, EcMinC interacts with EcMinD to be associated with membrane and to inhibit FtsZ polymerization at the polar region [8]. These data suggest that EcMinC may interact with AtMinD in chloroplasts. Figure 4 Localization of a chloroplast-targeted EcMinC-GFP in Arabidopsis. (A to C) 35S-GFP transiently expressed in an Arabidopsis protoplast; (D to F) 35S-TP-GFP transiently expressed in Arabidopsis protoplasts; (G to I) 35S-TP-EcMinC-GFP transiently expressed in an Arabidopsis protoplast. All bars, 5 μm. To further confirm the interaction between AtMinD and EcMinC, we did a BiFC analysis based on the reconstitution of YFP fluorescence when nonfluorescent

N-terminal C646 manufacturer YFP (YFPN) and C-terminal YFP (YFPC) fragments are brought together by two interacting proteins in living plant cells. These two proteins were fused with a oxyclozanide chloroplast transit peptide and a part of YFP and transiently coexpressed in Arabidopsis protoplasts (Figure 5). AtMinD was tested by being fused with either YFPN or YFPC tag at the C-terminus for the interaction with EcMinC which has an YFPC or YFPN at the C-terminus (Figure 5E and 5F). In both cases, a strong YFP signal was detected at puncta in chloroplasts in contrast to the negative controls (Figure 5A, B and 5C). It has been shown that AtMinD can self interact by FRET analysis [20] and BiFC assay [26]. Here as a positive control, AtMinD

self-interacts at puncta in chloroplasts by BiFC assay (Figure 5D). Overall, our data strongly suggest that AtMinD can interact with EcMinC. Figure 5 Interactions of EcMinC and AtMinD examined by BiFC assay in Arabidopsis protoplasts. (A) coexpression of 35S-YFPN and 35S-YFPC; (B) 35S-TP-EcMinC-YFPN and 35S-YFPCcoexpression; (C) 35S-AtMinD-YFPN and 35S-YFPCcoexpression; (D) 35S-AtMinD-YFPN and 35S-AtMinD-YFPCcoexpression; (E) 35S-AtMinD-YFPN and 35S-TP-EcMinC-YFPC coexpression; (F) 35S-TP-EcMinC-YFPN and 35S-AtMinD-YFPCcoexpression. Bars, 5 μm. It is interesting that AtMinD can still recognize EcMinC. However, no MinC homologue has been found in Arabidopsis and other higher plants yet. There are at least two possibilities. First, there are a lot of differences between chloroplasts and cyanobacteria in their structure, composition and function etc.

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