Of the plastidic FtsHs, FtsH1, 2, 5, and 8 are localized in the thylakoid membrane. These members are the most abundant FtsH proteases and extensively studied [44]; they form hetero-hexameric complexes, in which FtsH1 and FtsH5 (Type A) and FtsH2 and FtsH8 (Type B) can partially substitute for each other [45]. A threshold in the amount of type A and B subunits was postulated to determine the proper function and development of chloroplasts and thylakoid membrane [46,47,48,49]. This thylakoid located protease complex plays a vital role in the degradation and assembly of the Photosystem II reaction center protein D1 and other transmembrane subunits of the photosynthetic machinery. Mutants lacking FtsH2/VAR2 or FtsH5/VAR1 show strongly or slightly variegated leaves, respectively [50,51]. Functional loss of, e.g., FtsH2 results in upregulation of other FtsH proteins in the green leaf sectors to maintain proper function and development of the chloroplasts [47,50,52]. FtsH6 is also localized in the thylakoid membrane. It is essential for thermotolerance and thermomemory in seedlings [53], while no phenotype was observed in adult plants when grown in semi-natural outdoor conditions [54].

The other plastidic FtsH enzymes are believed to be localized in the chloroplast envelope [19]. Deleting FtsH7 and 9 does not result in any obvious phenotype [53], and the proteases are not required for PSII repair [55]. FtsH11 is crucial for growth in long photoperiods [40] and thermotolerance [56,57]. FtsH12 was co-immuno-precipitated in a complex with FtsHi1, 2, 4, 5 and NAD-dependent malate dehydrogenase (MDH) and shown to be involved in protein import [58,59]. In addition to FtsHi1, 2, 4, and 5, even FtsHi3 belongs to the five plastidic FtsH homologues, which are incapable of proteolysis in Arabidopsis. The FtsHi enzymes either have a mutation in their HEXXH motif (FtsHi1, 2, 4, and 5), or the entire motif is missing (FtsHi3) [18,26]. Compared to AtFtsHi1, 2, 4, and 5, FtsHi3 contains a very short C-terminal domain. Interestingly, FtsHi3 also has undergone a domain swap: the whole M41 domain is located at the N-terminal instead of at the C-terminal to the AAA⁺ domain [26]. Comparing the domain organization of AtFtsHi3 with AtFtsHi1, AtFtsH7, 9, 12 (Figure 1), also AtFtsH7/9 contain this “peptidase M41 FtsH extracellular” domain N-terminal to the AAA⁺ domain, which is additional to their protease domain located in the C-terminal to the AAA⁺ domain. This additional domain is not present in other FtsHs or FtsHis. Whether the N-terminal “peptidase M41 FtsH extracellular” domain of FtsH7, FtsH9, and FtsHi3 enables these enzymes to form a common complex with a specific function remains to be shown. Three independent pre-protein translocating models (pSSU-TEV-protein A, pL11Flag-TEV-Protein A, pLHCP-TEV-protein A) suggested FtsHi3 to form a 1-MD complex separate from the FtsH12/FtsHi1,2,4,5/MDH complex [58] and different to the 1-MD TIC complex [60]. The identity of other components in this complex is unknown. FTSHi3 is not co-expressed with the tight cluster of FTSH12/FTSHi1, 2, 4, 5, but instead with a gene encoding OTP51 [26,58,59]. This pentatricopeptide repeat protein is required for the splicing of group IIa introns and impacts photosystem I and II assembly [61]. The tight co-expression with FTSHi3 indicates a common function of OTP51 and FtsHi3; therefore, OTP51 is another hypothetical complex partner.

2.1.2. FtsH Proteases Located in the Chloroplast Envelope

The other plastidic FtsH enzymes are believed to be localized in the chloroplast envelope [19]. Deleting FtsH7 and 9 does not result in any obvious phenotype [53], and the proteases are not required for PSII repair [55]. FtsH11 is crucial for growth in long photoperiods [40] and thermotolerance [56,57]. FtsH12 was co-immuno-precipitated in a complex with FtsHi1, 2, 4, 5 and NAD-dependent malate dehydrogenase (MDH) and shown to be involved in protein import [58,59]. In addition to FtsHi1, 2, 4, and 5, even FtsHi3 belongs to the five plastidic FtsH homologues, which are incapable of proteolysis in Arabidopsis. The FtsHi enzymes either have a mutation in their HEXXH motif (FtsHi1, 2, 4, and 5), or the entire motif is missing (FtsHi3) [18,26]. Compared to AtFtsHi1, 2, 4, and 5, FtsHi3 contains a very short C-terminal domain. Interestingly, FtsHi3 also has undergone a domain swap: the whole M41 domain is located at the N-terminal instead of at the C-terminal to the AAA⁺ domain [26]. Comparing the domain organization of AtFtsHi3 with AtFtsHi1, AtFtsH7, 9, 12 (Figure 1), also AtFtsH7/9 contain this “peptidase M41 FtsH extracellular” domain N-terminal to the AAA⁺ domain, which is additional to their protease domain located in the C-terminal to the AAA⁺ domain. This additional domain is not present in other FtsHs or FtsHis. Whether the N-terminal “peptidase M41 FtsH extracellular” domain of FtsH7, FtsH9, and FtsHi3 enables these enzymes to form a common complex with a specific function remains to be shown. Three independent pre-protein translocating models (pSSU-TEV-protein A, pL11Flag-TEV-Protein A, pLHCP-TEV-protein A) suggested FtsHi3 to form a 1-MD complex separate from the FtsH12/FtsHi1,2,4,5/MDH complex [58] and different to the 1-MD TIC complex [60]. The identity of other components in this complex is unknown. FTSHi3 is not co-expressed with the tight cluster of FTSH12/FTSHi1, 2, 4, 5, but instead with a gene encoding OTP51 [26,58,59]. This pentatricopeptide repeat protein is required for the splicing of group IIa introns and impacts photosystem I and II assembly [61]. The tight co-expression with FTSHi3 indicates a common function of OTP51 and FtsHi3; therefore, OTP51 is another hypothetical complex partner.

3. Pseudo-Proteases with an Important Enzymatic Activity

In addition to being pseudo-proteases, the AAA⁺ domain of FtsHis is intact and—based on the seed lethality of many FtsHi mutants—highly important for their activity, plastid, and overall plant development. Four out of the five AtFtsHi members have been demonstrated to form an inner envelope-bound heteromeric AAA⁺ (ATPase associated with diverse cellular activities) ATPase complex. This complex consisting of FtsH12/FtsHi1,2,4,5/pdNAD-MDH was found to be involved in ATP-driven protein import across the chloroplast envelope [58,59,62,63]. Even Ycf2 was observed being part of this 2 MDa complex using transgenic lines overexpressing FTSH12 [58]. Still, the protein could not be detected in complexes isolated from wild-type and tic56-3 plastids using a combination of native gel electrophoresis and protein quantification [64] and neither after pull-down of FtsH12 using its native promoter [65]. Kikuchi and coworkers [57] determined the super-complex Ycf2-FtsH12-FtsHi1,2,4,5-pdNAD-MDH physically to interact with TIC components such as Tic214 (Ycf1), Tic100, and Tic56 as well as with the pre-protein translocation components Toc75 and Toc159 [59]. In this complex, neither pdNAD-MDH activity [59] nor FtsH12 proteolytic activity [57] are required; an FtsH12 (H769Y) mutant developed normal chloroplasts with functional pre-protein import abilities.

The finding of ATP-driven protein import across the chloroplast membrane by an FtsH12/FtsHi1,2,4,5/pdNAD-MDH complex has steered an intense debate [66,67] on the importance of the long-accepted chloroplast protein import machinery, i.e., Tic110 and Tic40 forming a common translocon in the inner chloroplast membrane and recruiting the stromal chaperones Hsp93/ClpC1, cpHsp70, and Hsp90C [67]. If indeed the FtsH12/FtsHi complex plays the main role in protein import into the chloroplast [67] remains to be shown. The absence of this complex in most monocots (see Section 4) as well as its lower impact in adult plants (see Section 5) rather point to a specific function during chloroplast development in dicotyledons. We refer th