Electron Tomography Analysis of Thylakoid Assembly and Fission in Chloroplasts of a Single-Cell C4 plant, Bienertia sinuspersici

Bienertia sinuspersici is a single-cell C4 plant species of which chlorenchyma cells have two distinct groups of chloroplasts spatially segregated in the cytoplasm. The central vacuole encloses most chloroplasts at the cell center and confines the rest of the chloroplasts near the plasma membrane. Young chlorenchyma cells, however, do not have large vacuoles and their chloroplasts are homogenous. Therefore, maturing Bienertia chlorenchyma cells provide a unique opportunity to investigate chloroplast proliferation in the central cluster and the remodeling of chloroplasts that have been displaced by the vacuole to the cell periphery. Chloroplast numbers and sizes increased, more notably, during later stages of maturation than the early stages. Electron tomography analyses indicated that chloroplast enlargement is sustained by thylakoid growth and that invaginations from the inner envelope membrane contributed to thylakoid assembly. Grana stacks acquired more layers, differentiating them from stroma thylakoids as central chloroplasts matured. In peripheral chloroplasts, however, grana stacks stretched out to a degree that the distinction between grana stacks and stroma thylakoids was obscured. In central chloroplasts undergoing division, thylakoids inside the cleavage furrow were kinked and severed. Grana stacks in the division zone were disrupted, and large complexes in their membranes were dislocated, suggesting the existence of a thylakoid fission machinery.

In Bienertia-type SCC4 plants, chlorenchyma cells have central chloroplasts (CCs) and peripheral chloroplasts (PCs). Bienertia CCs are located in a tightly packed central cytosolic compartment (CCC). PCs are dispersed around the outer edges of the cell near the plasma membrane. PCs generate a C4 organic acid from atmospheric CO 2 , and the organic acid is decarboxylated in mitochondria in the CCC to supply CO 2 to CCs. In contrast to the NADP-ME type in maize, Bienertia operates in NAD-ME type C4 photosynthesis. The CO 2 -capturing PCs have fewer grana stacks than the Rubisco-containing CCs because of CCs' requirements for reducing power as well as ATP 2,3 .
Biogenesis of SCC4 systems is of interest to plant biologists due to their unique cytoplasmic organization and regulation of photosynthetic genes 6 . Young Bienertia chlorenchyma cells have uniform chloroplasts operating in C3 photosynthesis and their cytoplasm is not partitioned 7 . As the chlorenchyma cells mature, vacuoles enlarge to enclose chloroplasts and mitochondria in the cell center and chloroplasts excluded from CCC become PCs 8 . In mature Bienertia SCC4 cells, CCs and PCs contain distinct sets of proteins for C4 photosynthesis, and they exchange small molecules through channels composed of cytoplasmic strands. Rubisco large subunit gene in the plastid genome are transcribed specifically in CCs, indicating that transcription in CCs is regulated differently from that in PCs 7 . A mechanism for selective targeting of chloroplast proteins encoded in the nuclear genome to one of the two chloroplast types has been characterized recently. The N-terminal signal peptides of proteins destined for PCs have two components, one that facilitates general entry into the chloroplast and a second one that inhibits import into CCs 9,10 . In agreement with their macromolecular compositions, CCs and PCs exhibit differential ultrastructural characteristics, but there have been no detailed morphometric analyses to show how CCs and PCs diverge from a homogenous pool of chloroplasts in young in Bienertia chlorenchyma cells.
Plastids divide via binary fission, and hourglass-shaped dividing proplastids have been observed in electron microscopy (EM) imaging of shoot apical meristem cells 11 . Constriction of the plastid envelope membranes is mediated by two ring complexes, one in the stroma, termed Z-ring, and the other in the cytosol consisting of a dynamin-related protein 12 . The thylakoid membrane is densely populated with massive photosynthetic complexes, and some of them constitute close-packed two-dimensional arrays. It seems a daunting task to bisect piles of thylakoid membranes in grana stacks for chloroplast division but almost none is known about thylakoid fission. However, it has been elusive how thylakoids are partitioned into two daughter chloroplasts during division 13 .
A distinctive feature of the Bienertia chloroplast is that large numbers of CCs are packed in the central cytosol; these chloroplasts multiply as chlorenchyma cells develop 7,8 . The Bienertia CC cluster provides a unique opportunity to examine thylakoids in dividing chloroplast with transmission electron microscopy (TEM)/electron tomography (ET). Most plastid division in plants happens in meristematic cells in which proplastids have primitive thylakoids. It is challenging to find dividing chloroplasts by TEM because chloroplasts in the leaf divide less frequently than proplastids in the meristematic zone, and leaf cells are large, highly vacuolated 11,14 . It is critical for TEM analysis to acquire unambiguous micrographs of dividing chloroplasts repeatedly in leaf samples of which subcellular structures are preserved close to their native states. The CC division occurs in a restricted volume in the cell center, making it easy to identify many dividing chloroplasts under TEM and capture images of their thylakoids. Furthermore, well-developed thylakoids appear in chlorenchyma cells of young Bienertia leaves 15 , facilitating high-pressure freezing fixation of the leaf samples.
ET imaging of cryofixed chloroplast has been an essential approach to determine 3D architectures of the photosynthetic organelle as well as macromolecular structures of its constituents that are close to their native states [16][17][18][19] . Taking advantage of these advanced microscopy techniques, we characterized the gradual modifications of thylakoid architectures in CCs and PCs as SCC4 is established in Bienertia chlorenchyma cells. We were able to delineate thylakoid growth from inner membrane invaginations that expand over planar thylakoid surfaces to add to a layer in the grana stack. Additionally, the concentrated chloroplasts at the central cytoplasm facilitated EM analyses of chloroplast division. Thylakoid division involved distortion of grana stacks at the constricted site before severing, and displacement of PSII components from the deformed stacks.

Results
Morphometric analysis of chloroplasts in maturing Bienertia chlorenchyma cells. In order to monitor the maturation process of dimorphic chloroplasts in Bienertia sinuspersici, we examined chloroplasts in chlorenchyma cells at 1 st stage, 2 nd stage, 3 rd stage, and the mature stage as defined in Park et al. 8 using confocal laser scanning microscopy and TEM. The 1 st stage and 2 nd stage cells were sampled from leaves less than 0.3-cm long, 3 rd stage cells from leaves 0.4-cm to 0.5-cm long, and mature stage cells from the tip region of leaves 1.5cm to 2.0-cm long (Fig. 1A). In isolated mature chlorenchyma cells, two groups of chloroplasts were observed: densely packed chloroplasts in the central cytosol and chloroplasts scattered in the cell periphery (Fig. 1B).
The 1 st stage cells were spherical, and their cytoplasms were occupied mostly by chloroplasts (Fig. 1C). Vacuoles divided the cytosol into central and peripheral regions in older cells, but no large vacuoles were observed in 1 st stage cells (Fig. 1D-F). Vacuole development was discerned from 2 nd stage, separating some chloroplasts to the cell periphery, and by the 3 rd stage, chlorenchyma cells had elongated to take on elliptical shapes and vacuoles segregated PCs from CCs. Cells at the mature stage grew into a pill shape with a corresponding increase in the size and number of chloroplasts ( Fig. 1H-M). In TEM micrographs, PCs appear oppressed in the thin cytosol between the vacuole and the plasma membrane (Fig. 1M). Numerous mitochondria were intermixed with chloroplasts in the CCC (Fig. 1K-M).
We were able to estimate cell sizes, cell numbers, and sizes of chloroplasts in the cell at the four stages from confocal laser scanning microscopy data (Fig. 1G)  electron tomography analysis of thylakoid assembly. It has been shown by TEM that thylakoid organizations of the CCs and PCs are dissimilar in mature Bienertia chlorenchyma cells 7 . We investigated the biogenesis of dimorphic chloroplasts using electron tomography (ET), which allowed three dimensional morphometric analysis of membranous compartments 20 . No ultrastructural differences were apparent in the thylakoid architectures of the two types of chloroplasts in 2 nd stage cells, but in 3 rd stage chloroplasts, we were able to observe differential architectures in the thylakoids that became even more apparent in mature cells ( Fig. 2A-L). The 3 rd stage CCs became enriched with grana stacks (2M, green brackets) and short stroma thylakoids connecting the stacks were seen. Grana stacks widened in PCs without obtaining additional layers, making it difficult to identify discrete stacks (Fig. 2N). By the mature stage, the two types of chloroplasts exhibited the structural dimorphism reported previously 15 . Mature CCs were ovoid and grana stacks and unstacked thylakoids were well differentiated in their stroma. Their grana stacks had 2-5 layers and some had as many as 10-11 layers (Fig. 2C,F,O,Q). Mature PCs were flattened into a discus-like shape which appeared as a rod in 2D images (Fig. 2I,L). The thylakoid www.nature.com/scientificreports www.nature.com/scientificreports/ composition PCs was remarkably skewed toward unstacked stroma thylakoids (Fig. 2P,Q), although there were grana stacks with 2-3 layers (Fig. 2P, green brackets).
We generated 3D models of thylakoid membranes and envelope membranes in the tomograms ( Fig. 2D-F,J-L) and calculated volume ratios of thylakoids to their chloroplasts. Relative volumes of thylakoids increased in both types of chloroplasts as they matured (Fig. 2R), indicating that thylakoids proliferate more rapidly than chloroplasts enlarge. Given that chloroplast sizes increased most between the 3 rd stage and the mature stage (Fig. 1G), we inferred that thylakoid biogenesis is most active in 3 rd stage chloroplasts. From the 3 rd stage, volumes of thylakoids in CCs were larger than those in PCs (Fig. 1G).
Invaginations from the inner envelope membrane and thylakoid assembly. To investigate how thylakoids assemble in the Bienertia chloroplasts, we examined electron tomograms from CCs of 3 rd stage cells, the stage of fastest growth. Round membrane outlines were frequently discerned in the stroma close to the envelope and some of them were connected to the envelope membranes (Fig. 3A,B, arrowheads). Similar invaginations were observed in proplastids of cotyledon cells of germinating Arabidopsis thaliana seedlings (Liang et al. 21 ).
We generated 3D models of membrane elements in the vicinity of the ingrowths including the existing thylakoid network and IEM to better understand their relationship (Fig. 3A-D). It is evident that the volume of thylakoid membrane increases in growing chloroplasts. When we arranged IEM invaginations according to their surface areas, we discerned vesicle-shaped ingrowths (Fig. 3E, Movie S1) and more elaborate ingrowths that seemed to have formed by lateral fusion of isolated ingrowths (Fig. 3G, Movie S3). These thylakoid precursors appeared to expand over a grana stack when it encounters its top surface (Fig. 3H, Movie S4). Ingrowths in close proximity with stroma thylakoid (Fig. 3F, arrowhead, Movie S2) were also observed, suggesting that this may constitute a membrane contact site between the IEM and peripheral membranes of the granum. We were able to identify discrete membrane compartments overlaying a thylakoid that seem to have separated from IEM (Fig. 3I, Movie S5), suggesting that the IEM ingrowths can be detached before they merge with the thylakoid system. However, no free-floating vesicles in the stroma were detected.

Division of chloroplasts within an existing thylakoid network. The number of chloroplasts increased
during the Bienertia chlorenchyma cell development (Fig. 1G, left panel), and chloroplasts of chlorenchyma cells as early as 2 nd stage accumulate grana stacks (Figs. 1 and 2). Grana stacks are packed with large protein complexes of the electron transport chain embedded in the thylakoid membrane, and these stacks could impede separation of daughter chloroplasts. To understand how grana stacks are partitioned in dividing chloroplasts, we examined 2 nd stage and 3 rd stage Bienertia cells with electron microscopy/tomography.
Dividing CCs were frequently observed in the central cytoplasmic regions of 2 nd stage and 3 rd stage cells where dozens of chloroplasts are clustered (Fig. 4A). Very few dividing chloroplasts were seen in the cell periphery under TEM because PCs are rare and scattered over large areas. Dividing chloroplasts were elongated and peanut-shaped due to constriction near the center (arrowheads in Fig. 4A). Interestingly, thylakoids appeared sharply kinked at the division plane at the constricted site (Fig. 4B,C). Electron tomography imaging confirmed that the stack architecture was disrupted. Furthermore, some thylakoids were disjoined as if they had been severed (Fig. 4C,D, arrowheads).
We examined dividing chloroplasts in cryofixed Arabidopsis cotyledons to test whether the thylakoid remodeling in dividing Bienertia chloroplasts is conserved. Thylakoids began to fold into 2 or 3 layers at 60 hours after imbibition (HAI), and grana stacks constituted the majority of thylakoids in chloroplasts by 120 HAI as previously reported (Liang et al. 21 ). It was more challenging to detect dividing chloroplasts in 120 HAI Arabidopsis cotyledon cells by TEM than it was in Bienertia cells.
As in dividing chloroplasts of Bienertia, thylakoid membranes in the division zone were highly twisted in 120 HAI Arabidopsis chloroplasts (Fig. 4E-H). Electron-dense particles of approximately 10 nm constituting a 2D crystalline array were discerned in appressed membranes of grana stacks (Fig. 4I,J), but these particles were not observed in the kinked thylakoid membranes (Fig. 4K,L). We hypothesize that these particles that have dislocated from the fission sites correspond to PSII. To test this, we localized a subunit of the oxygen-evolving complex of PSII, PsbP, in 120 HAI Arabidopsis cotyledon cells using immunogold particles. In dividing chloroplasts, PsbP-specific gold particles were absent from the disrupted thylakoids, indicating that the thylakoid remodeling in dividing chloroplasts involves PSII removal (Fig. 4M,N).
Meristem cells have proplastids, and they do not have extensive grana stacks 22 . We examined dividing proplastids to determine whether their prothylakoids are severed when the ring complexes at the envelope squeeze the envelope membranes. In consecutive sections of an Arabidopsis meristem cells where two daughter proplastids are about to separate, we observed a connecting neck and a tubular prothylakoid (Fig. 4O). This observation indicates that prothylakoids are not disconnected in preparation for the shrinking envelope membranes probably because they do not interfere with plastid constriction.

Discussion
We analyzed development of dimorphic chloroplasts in chlorenchyma cells of Bienertia sinuspersici with structural biology approaches. Our results indicate that thylakoids assemble through growth and fusion of inner membrane invaginations and that disjoining of thylakoids precedes constriction of the envelope membranes.   www.nature.com/scientificreports www.nature.com/scientificreports/ Our TEM and ET analyses indicated that the 3 rd stage is critical in the establishment of the Bienertia dimorphic chloroplasts. In 1 st stage and 2 nd stage cells, no significant ultrastructural variations were detected among chloroplasts. Thylakoids with 2 or 3 layers were abundant in both types of chloroplasts in these early stages. In CCs, beginning in the 3 rd stage, the number of layers per thylakoid stack increased and discrete stacks appeared. By contrast, thylakoids spread laterally in PCs, and they lost the layered architecture. That protoplasts from "young cells" are capable of selective protein targeting to the PC was demonstrated by Wimmer et al. (2017) 9 ; these authors took advantage of this targeting to characterize mechanisms of PC-specific protein accumulation. Considering cell structure and size, 3 rd stage cells correspond to "young cells". It is likely that the morphological variations in the thylakoids in 3 rd stage cells result from targeting of proteins involved in thylakoid stacking to CCs and their exclusion from PCs; these proteins include those that stabilize the stack margins such as LHCB subunits and CURT1 family proteins 18,23,24 . Lateral stretching of thylakoids ( Fig. 2I-L) and lack of grana-forming proteins in 3 rd stage PCs could lead to their distinct thylakoid architecture in the mature stage. Offermann et al. (2015) isolated central and peripheral chloroplasts to measure relative abundances of PSII and PSI subunits in the chloroplasts using mass spectrometry analysis 6 . In agreement with the preferential grana stacking in CCs, LHCB proteins mediating membrane stacking are more abundant (up to two-fold) in CCs than PCs.
Thylakoid assembly is the hallmark of chloroplast biogenesis 25,26 . Conversions of proplastids and etioplasts into chloroplasts have been characterized by ET, and these studies led to our current understanding of construction of the photosynthetic apparatus 21,22,27 . We provide evidence for a mechanism of thylakoid assembly involving IEM invaginations that enlarge and become integrated with existing thylakoids. They also formed contact sites with membranes of planar thylakoids (Fig. 3). In Arabidopsis proplastids, thylakoid assembly takes place throughout the stroma in a linear order 21,27 . By contrast, the Bienertia chloroplast has an elaborate thylakoid network in the stroma and the construction process is confined to the vicinity of the envelope membrane (within 100 nm from IEM). Given that we did not identify vesicle-like carriers in the stroma, roles of vesicle carriers reported earlier from studies in higher plants 28 seems limited in the Bienertia thylakoid assembly.
The intermediate structures derived from IEM resemble what was proposed in Bastien et al. 29 . We have detected IEM ingrowth, the formation of flattened invaginations, and the development of contact sites between IEM and planar thylakoids (Fig. 3). These membrane junctions are reminiscent of the endoplasmic reticulum (ER) -chloroplast contact sites. Galactolipids monogalactosyldiacylglycerol (MGDG) and digalactosyldiacylglycerol (DGDG) comprise >75% of the thylakoid membrane and IEM. The rest is composed of two anionic lipids, sulfoquinovosyldiacylglycerol (SQDG) and phosphatidylglycerol (PG) 30 . These four lipids are partly or entirely transferred from ER. The lipid compositions of IEM and thylakoid membrane are broadly similar. Expansion of thylakoid membranes that cannot directly interact with IEM may acquire lipid molecules through the IEM-thylakoid contact sites.
FZL is a dynamin-related protein targeted to the chloroplast. Arabidopsis mutant lines in which FZL is inactivated have fragmented thylakoids, suggesting that FZL is involved in thylakoid membrane fusion 21,31 . Recently, Findinier et al. demonstrated that FZL in Chlamydomonas mediates thylakoid membrane fusion using an ingenious biochemical assay 32 . FZL localizes to thylakoid margins suggesting that grana stacks and stroma lamellae are interlinked through their periphery. FZL orthologs of Bienertia could contribute to combining the thylakoid precursors derived from IEM to margins of grana stacks or thylakoid lamellae.
In dividing chloroplasts of Bienertia chlorenchyma cells as well as Arabidopsis cotyledon cells, kinked thylakoid membranes were seen along the midline connecting the division furrows (Fig. 4). Peanut-shaped chloroplasts that appear to go through fission have been documented before and thylakoids constricted in the neck region have been observed in several land plant species 33,34 . But the unusual thylakoid architecture that we have observed in this study has not been reported previously. We infer that chemical fixation may fail to preserve the intriguing U-shaped thylakoids. It has been demonstrated that high-pressure freezing and subsequent freeze substitution can capture transient and fragile subcellular structures in plant cells that conventional TEM protocols cannot 35,36 . The thylakoid remodeling and splitting visualized in our study benefited from the congregated chloroplast arrangement in growing Bienertia chlorenchyma cells and the improved sample preservation methods employed for electron microscopy 37 . It was possible to discern dividing chloroplasts in 120 HAI Arabidopsis cotyledon cell samples, although these were extremely rare, and we examined the displacement of thylakoid membrane proteins in the samples. However, we failed to identify dividing chloroplasts in true leaf cells of Arabidopsis seedlings.
of electron-dense complexes in the kinked region (blue dashed oval) as compared to stacked regions around it (green arrows). (M,N) Electron micrograph of a dividing Arabidopsis chloroplast. PsbP, a subunit of PSII, was localized by immunogold labeling. Panel N is a higher magnification of the boxed area of panel M showing immunogold particles (green arrow heads, 15 nm gold particles). The particles are absent in the squeezed region (blue oval). St: starch particle. Scale bars in N = 500 nm (O) Three consecutive TEM sections (1/3-3/3) of an Arabidopsis meristem cell showing a dividing proplastid. The two daughter plastids are joined via a narrow isthmus (cyan arrowheads in the middle panel). A thin tubule is seen through it (blue arrows). Scale bar = 500 nm. (P) Model of the thylakoid fission [1] A chloroplast ready to divide; indicated are inner and outer envelope membranes (grey), thylakoid membranes (green), photosystem II (PSII) complexes (black squares), and the plane of division (red dotted line). [2] The thylakoid membranes are rearranged as they are 'pinched' along the plane of division (red arrowheads) as seen in E and F. PSII complexes are dislocated from the plane of division. The inner (blue dots) and outer (orange dots) division rings begin squeezing the envelope membranes. [3] The thylakoid severing is complete before the division rings separate the chloroplast as seen in (A,B). [5] Two daughter chloroplasts are formed from the division of the mother chloroplast. www.nature.com/scientificreports www.nature.com/scientificreports/ Components of the plastid division machinery have been identified and molecular mechanisms of their function have been characterized 38 . Two ring complexes, the DRP5B ring on OEM and the Z-ring inside IEM, assemble at the midzone of a dividing chloroplast to constrict the envelope membrane [39][40][41] . Linker complexes connecting the two rings on the opposite sides of the envelope regulate formation and contraction of the rings 42 . However, almost no information about thylakoid fission is available 13 . Based on our observations, we speculate that the thylakoid severing machinery bends thylakoid membranes and disrupts the array of PSII-LHCB complexes initiating their relocation, probably by exerting forces (Fig. 4P). Given that thylakoid cutting occurs precisely at the cleavage plane, it is conceivable that assembly and operation of the thylakoid division machinery is coordinated with those of the ring complexes. Because of the distance between the two apparatuses, it is puzzling how the contractile ring complexes at the envelope membranes communicate with the thylakoid division machinery in the stroma. The chloroplast Min system controls position of Z-ring formation and the inner membrane ring seems to trigger subsequent assembly of the linker and outer membrane ring complexes 43 . Establishment of the thylakoid fission machinery could be regulated by the Z-ring. Alternatively, the Min system might control assembly and activation of the thylakoid disjoining directly.
conclusions Bienertia sinuspersici, a single-cell C4 plant species, is a useful model organism for studying the development of dimorphic chloroplasts and the selective targeting of nucleus-encoded plastid proteins to central and peripheral chloroplasts. Through light and electron microscopy analyses of Bienertia chloroplasts, we delineated the assembly process of thylakoid membranes in a growing chloroplast, observed the gradual gain of grana stacks in the central chloroplasts and their loss in peripheral chloroplasts, and the fission of grana thylakoids in dividing chloroplasts. The observations of thylakoid membranes and the division of chloroplasts presented here diverge from what has been seen in those of proplastids, expanding our understanding of chloroplast biogenesis in higher plants. These observations were made possible by state-of-the-art cryo-preservation and three-dimensional electron microscopy techniques, and investigations of plastids employing these tools in other species are well warranted. Mitochondria are vital in the NAD-ME type C4 photosynthesis occurring in Bienertia leaf cells. Further work is needed to characterize the subgroups of mitochondria that associate with the tightly-packed CCs. The leaves were then cut and sized to different stages as shown in Fig. 1A. Arabidopsis seedlings were grown as described in Lee et al. 44 . Briefly, the seeds were germinated and grown on 0.75% phytoagar plates supplemented with ½ MS salt (0.5 g/l, pH 5.7) under continuous light at a photon flux density of 120 mol quanta m −2 s −1 in a growth chamber at 22 °C before their cotyledons were dissected for high-pressure freezing and electron microscopy experiments.
confocal laser scanning microscopy. Isolated chlorenchyma cells were examined using confocal laser scanning microscopes FluoView FV1000 (Olympus, Japan) & TCS SP5 II MP with SMD (Leica Microsystems, Germany) to assess their chlorophyll autofluorescence. Stacked images of the chloroplast in Fig. 1C-F were prepared using FV10-ASW Ver. 3.1 Viewer (Olympus, Japan) and other images were processed using ImageJ (LOCI, University of Wisconsin, USA).
High-pressure freezing, sample processing, electron microscopy, and electron tomography. High-pressure freezing, freeze substitution, resin embedding, and ultra-microtomy were performed as described 45 . Bienertia chlorenchyma tissue and Arabidopsis cotyledon tissue were dissected and rapidly frozen with an HPM100 high-pressure freezer (Leica Microsystems, Germany). Two different freeze-substitution protocols were used and processed in an EM AFS2 freeze-substitution machine (Leica Microsystems, Germany). For ultrastructural analysis, the samples were freeze-substituted at −80 °C for 72 h in 2% osmium tetroxide (OsO 4 ) dissolved in anhydrous acetone, and excess OsO 4 was removed by rinsing with precooled acetone. After being slowly warmed up to room temperature over 48 h, tissue samples were separated from planchettes and embedded in Embed-812 resin (Electron Microscopy Sciences, USA). For immunogold labelling samples, anhydrous acetone containing 0.25% glutaraldehyde and 0.1% uranyl acetate was used for freeze-substitution media at −80 °C for 72 h before being slowly warmed up to −45 °C where they were embedded with Lowicryl HM20 resin (Electron Microscopy Sciences, USA) and polymerized under ultraviolet light for 24 h at −45 °C.
The blocks were trimmed and sectioned into 100 nm sections using a diamond knife (Diatome, Switzerland) and an UC7 ultramicrotome (Leica Microsystems, Germany) onto slot grids (Electron Microscopy Sciences, USA) and examined with a Hitachi 7400 TEM (Hitachi-High Technologies, Japan) operated at 80 kV. For ultrastructural analysis, 250 nm thick sections were collected on formvar-coated copper slot grids (Electron Microscopy Sciences, USA) and stained with 2% uranyl acetate in 70% methanol followed by Reynold's lead citrate (Electron Microscopy Sciences, USA). A 200-kV Tecnai F20 intermediate voltage electron microscopy (Thermo-Fischer, USA) was used to collect tilt series from ±60 at 1.5° intervals in brightfield TEM mode and from ±51° at 1.5° intervals in scanning transmission electron microscopy (STEM) mode. For dual-axis tomography analysis, tilt