Journal of Structural Biology 184 (2013) 203–211 Contents lists available at ScienceDirect Journal of Structural Biology journal homepage: www.elsevier.com/locate/yjsbi 3-D analysis of dictyosomes and multivesicular bodies in the green alga Micrasterias denticulata by FIB/SEM tomography q Gerhard Wanner a, Tillman Schäfer a, Ursula Lütz-Meindl b,⇑ a b Ultrastructural Research, Faculty of Biology, Ludwig-Maximilians-University, Munich, Großhadernerstr 2-4, D-82152 Planegg-Martinsried, Germany Plant Physiology Division, Cell Biology Department, University of Salzburg, Austria a r t i c l e i n f o Article history: Received 21 June 2013 Received in revised form 30 September 2013 Accepted October 2013 Available online 14 October 2013 Keywords: FIB/SEM tomography Dictyosomes Multivesicular bodies ER Micrasterias denticulata TEM a b s t r a c t In the present study we employ FIB/SEM tomography for analyzing 3-D architecture of dictyosomes and formation of multivesicular bodies (MVB) in high pressure frozen and cryo-substituted interphase cells of the green algal model system Micrasterias denticulata The ability of FIB/SEM of milling very thin ‘slices’ (5–10 nm), viewing the block face and of capturing cytoplasmic volumes of several hundred lm3 provides new insight into the close spatial connection of the ER–Golgi machinery in an algal cell particularly in z-direction, complementary to informations obtained by TEM serial sectioning or electron tomography Our FIB/SEM series and 3-D reconstructions show that interphase dictyosomes of Micrasterias are not only closely associated to an ER system at their cis-side which is common in various plant cells, but are surrounded by a huge ‘‘trans-ER’’ sheath leading to an almost complete enwrapping of dictyosomes by the ER This is particularly interesting as the presence of a trans-dictyosomal ER system is well known from mammalian secretory cells but not from cells of higher plants to which the alga Micrasterias is closely related In contrast to findings in plant storage tissue indicating that MVBs originate from the transGolgi network or its derivatives our investigations show that MVBs in Micrasterias are in direct spatial contact with both, trans-Golgi cisternae and the trans-ER sheath which provides evidence that both endomembrane compartments are involved in their formation Ó 2013 The Authors Published by Elsevier Inc All rights reserved Introduction The plant Golgi apparatus positioned at the cross-road between the secretory-biosynthetic and the endocytotic-vacuolar pathway fulfills a great number of different functions ranging from polysaccharide synthesis, protein glycosylations, and transfer, sorting of products, regulation of vesicle trafficking up to vacuole formation and participation in degradation processes (among numerous others, see reviews by Faso et al (2009), Hawes and Satiat-Jeunemaitre (2005)) As synthesis site for most constituents of the cell wall, it is central in plant development and plays an important role in response to environmental impact The diverse functions of the Golgi apparatus are reflected in the unique morphology and structural integrity of the numerous motile dictyosomes of a plant cell (Hawes, 2005) While spatially and functionally tightly associated q This is an open-access article distributed under the terms of the Creative Commons Attribution-NonCommercial-No Derivative Works License, which permits non-commercial use, distribution, and reproduction in any medium, provided the original author and source are credited ⇑ Corresponding author Address: Cell Biology Department, Plant Physiology Division, University of Salzburg, Hellbrunnerstrasse 34, 5020 Salzburg, Austria E-mail addresses: wanner@lrz.uni-muenchen.de (G Wanner), tillman.schaefer@ gmx.de (T Schäfer), ursula.meindl@sbg.ac.at (U Lütz-Meindl) to the ER from where they are supplied with proteins and lipids, the flattened closely attached cisternae of a dictyosome usually display clear cis–trans-polarity Cis-, median- and trans-cisternae of a Golgi stack are involved in different steps of product processing and the tubular-reticular trans-Golgi network (TGN) acts as a sorting station that marks outgoing cargo for its destination and also holds the role of an early endosome (Hwang and Robinson, 2009; Staehelin and Moore, 1995; Viotti et al., 2010) The early endosome is the first compartment that receives cargo endocytosed from the plasma membrane (Otegui and Spitzer, 2008) Via different intermediate stages it may then mature to the late endosome which is frequently named multivesicular body (MVB) MVBs are essential for membrane recycling back to the TGN, may act as constituents of the degradation pathway ending up in the vacuole (Lam et al., 2007; Otegui and Spitzer, 2008; Robinson et al., 2008; Tanchak and Fowke, 1987) or may even be involved in the formation of autophagosomes (for references see below) By means of three-dimensional high-voltage electron microscopy early studies by Marty (1978, 1999) provided evidence that the TGN acts as starting point for generation of vesicle like provacuoles which develop to tubular prevacuoles by microinvagination of their membranes (see also Bassham et al (2006)) Provacuoles, prevacuoles or prevacuolar compartments are regarded as 1047-8477/$ - see front matter Ó 2013 The Authors Published by Elsevier Inc All rights reserved http://dx.doi.org/10.1016/j.jsb.2013.10.003 204 G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 Fig.1 (a), and (b) Different 3-D views of the trans-side of a dictyosome of M denticulata reconstructed from FIB/SEM series Cisternal rims are lacerated, outermost-transcisterna are shorter than others and undulated Secretory vesicles (grey) are connected to edges of trans-cisternae From red to green: cis- to trans-cisternae convergence point for either the endocytotic pathway or autophagy Provacuoles may sequester portions of cytoplasm by forming digitate extensions thus developing to early double-membrane autophagosomes lateron (Marty, 1978, 1999) Although the observations of Marty were based on chemically fixed tissue in which artificial membrane alterations cannot be excluded, the results are intriguing and deserve verification by means of a more reliable structure preservation technique More recent publications on high pressure frozen Nicotiana BY-2 cells (Tse et al., 2004) and Arabidopsis root tips (Scheuring et al., 2011) identified MVBs as prevacuolar compartments or provacuoles arising from one particular domain of the TGN and able to fuse with the vacuole in a non-vesicular way This process requires both TGN integrity and V-ATPase activity (Scheuring et al., 2011) In protein storage tissue of Arabidopsis embryos it has been found that two different populations of TGN derived vesicles containing either the storage protein or the processing enzymes, fuse into MVBs functioning as pre-vacuolar compartments (Otegui et al., 2006) Whereas numerous participants in these different degradation pathways have been identified, the structural transformation from the TGN into the MVB is still obscure This process however is crucial for both understanding the endocytotic and the degenerative pathway High pressure freeze fixation (HPF) for best structural preservation (Staehelin et al., 1990) combined with 3-D analysis such as electron tomography has been proved to be an excellent tool for getting insight into the development of dictyosomal or ER derived structures and their functions at high resolution (Donohoe et al., 2006; Hayashi-Nishino et al., 2009; Kang and Staehelin, 2008; Kang et al., 2011; Knott et al., 2008; Mogelsvang et al., 2004; Ylä-Anttila et al., 2009) Although the benefit of this technique for detailed structural analysis is undoubted, its limitations arise from the maximum thickness of the sections (400 nm; see Donohoe et al (2006)), from the maximum tilt angle of about 70° causing a ‘‘missing wedge’’ and from the relatively small volume (max $25 lm3) that can be calculated for the 3-D reconstructions The new technique of focused ion beam milling and viewing by field emission scanning electron microscopy (FIB/SEM) overcomes these problems and provides additional structural information by its ability of sectioning very thin slices (5–10 nm) parallel to the block face and by covering volumes of several hundreds of lm3 (Knott et al., 2008; Schroeder-Reiter and Wanner, 2009; Schroeder-Reiter et al., 2009, 2012) The resolution of FIB/SEM tomography does not yet reach the resolution of TEM in x/y but is close to it as clearly demonstrated in a recent publication (Villinger et al., 2012) In respect to analysis of dictyosomal derived membranes an additional advantage of this method is provided by the fact that several dictyosomes of a cell can be captured at the same time In the present study we employed this technique for analyzing the 3-D architecture of interphase dictyosomes of the algal model system Micrasterias denticulata (Meindl, 1993) and to obtain insight into structural connections between MVBs and endomembrane systems This alga is very well suited for such investigations as it possesses large dictyosomes with a constant average number of 11 cisternae throughout the cell cycle and their vesicular products during different developmental stages are well defined (Eder and Lütz-Meindl, 2008; Eder et al., 2008; Lütz-Meindl and Brosch-Salomon, 2000; Oertel et al., 2004) Moreover, numerous studies influencing the secretion pathway have provided information on the regulation of the secretory machinery (Lehner et al., 2009; Salomon and Meindl, 1996) Recently evidence has been obtained that Micrasterias is capable of performing autophagy and programmed cell death upon induction by abiotic stressors such as oxidative stress, high salinity or cadmium (Affenzeller et al., 2009a,b; Andosch et al., 2012) Coincidently with the occurrence of autophagy, environmental stress evokes severe structural alterations at dictyosomes (Affenzeller et al., 2009a,b; Darehshouri et al., 2008; Volland et al., 2011) Particularly cadmium induces a dose and time dependent complete disintegration of dictyosomes combined with an increase in the number of MVBs (Andosch et al., 2012) Although, like in other plant and animal systems, the ER contributes to autophagosome formation in Micrasterias there are several indications that MVBs may functions as sources for stress induced degeneration or even autophagosome formation as well (see above) Information on the structural origin of MVBs as provided by FIB/SEM tomography will therefore be important as a basis to understand stress induced degradation processes The present study shows that MVBs are frequently found in structural contact with both transGolgi cisternae and a ‘‘trans-ER’’ As Micrasterias is a member of Streptophyta belonging to the closest relatives of higher plants (Wodniok et al., 2011) we expect that the results obtained may be of general interest for plant cells and may also provide insight into evolutionary aspects of the first steps of degradation Materials and methods All chemicals were purchased from Roth (Karlsruhe, Germany) or Sigma–Aldrich (Vienna, Austria) unless stated differently 2.1 Cell cultures The unicellular freshwater green alga M denticulata was cultivated in a liquid Desmidiacean medium (Schlösser, 1982) in Erlenmeyer flaks at constant temperature of 20 °C and a light/dark regime of 14/10 h Cells were subcultured every 4–5 weeks To obtain defined interphase stages for FIB/SEM analyses, developmental stages were collected and were allowed to grow in nutrient solution for 48 h 2.2 High pressure freeze fixation for TEM and FIB/SEM tomography Interphase cells of M denticulata were high-pressure frozen and cryo-substituted following the protocol of Aichinger and G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 205 2.3 FIB/SEM tomography High pressure frozen and freeze substituted interphase cells of M denticulata were washed in acetone and transferred into propylenoxide and mixtures of epoxy resin/propylenoxide in ratios 1:3 and 1:2 and finally embedded in pure epoxy resin (see above) Cells were mounted on aluminum stubs covered with a thin layer of polymerized epoxy resin Blocks were trimmed with a LKB Pyramitome with glass knives that vertical faces allowed lateral milling of the cells by the FIB Tomographic datasets were obtained using the ‘‘slice and view’’ technique using a Zeiss Auriga 60 dual beam workstation (Carl Zeiss Microscopy, Oberkochen, Germany) For slicing with the focused ion beam, the conditions were as follows: 500 pA milling current of the Ga-emitter; with each step 7–10 nm of the epoxy resin was removed with the FIB SEM images were recorded with an aperture of 60 lm in the high current mode at 1.5 kV of the In-lens EsB detector with the EsB grid set to À1400 V Line averaging was performed The image pixel size was 5.3 Â 5.3 nm in x/y The dimensions of the recorded images were 2048 Â 1536 pixel According to the Nyquist criterion the resolution lies thus in the range of 12 nm The time to acquire one frame was 90s The slice and view process was repeated 500–1500 times to obtain the different datasets The contrast of the images was inversed, so that they appeared like a conventional bright field TEM image 2.4 Data processing and 3-D reconstruction Image stacking and alignment was performed with the open source software ImageJ (http://rsbweb.nih.gov/ij/index.html) Segmentation was performed using Amira Software (VSG; Visualization Sciences Group) Results Fig.2 FIB/SEM series of two dictyosomes of an interphase Micrasterias cell Transmost Golgi cisternae are shorter and involute respectively circular (arrows) ER cisternae present at both cis- and trans-side of the right dictyosome Framed area indicates vesicular contact between a trans-Golgi cisterna and the trans-ER Small secretory vesicles and large mucilage vesicles are visible around the left dictyosome 10 nm slices, every second image shown Lütz-Meindl (2005), Meindl et al (1992) In brief the cells were wrapped in cotton fibers to which they stick due to their surface mucilage, and frozen in a Leica EMPACT HPF device (Leica Microsystems, Austria) Freeze substitution was performed in a Leica EM AFS in 2% OsO4 and 0.05% uranyl acetate in anhydrous acetone Cells were embedded in epoxy resin (Agar low viscosity resin; Agar Scientific, Essex, UK) and sectioned on a Leica UC7 ultramicrotome for TEM 60–80 nm sections were mounted on formvar coated copper grids and investigated in a LEO 912 AB Omega TEM (Zeiss, Oberkochen, Germany) at 80 kV by using zero-loss energy filtering (Lütz-Meindl and Aichinger, 2004) Sections of all samples were viewed in TEM prior to analysis by FIB/SEM tomography Dictyosomes of Micrasterias interphase cells are mostly accumulated in the cell center around the nucleus or along the edges of the large chloroplast which covers each of the two semicells FIB/SEM slicing and 3-D analysis of the block-face images shows that the Golgi stacks consist of flat unfenestrated cisternae with lacerated rims (Fig 1a,b) Interconnections between the cisternae are frequently visible at the images series The outermost trans-cisterna is frequently shorter and more involute and differs in its structure from the others On FIB/SEM series (Fig 2) and TEM micrographs (Fig 3a,b) it appears chain-like constricted resulting in an undulated surface in the 3-D reconstruction (Fig 1b) During interphase the main products of dictyosomes in Micrasterias are large mucilage vesicles which origin from the edges of the outermost trans-cisternae and are also found accumulated around the dictyosomes (Fig 4, Suppl animation) Additionally smaller secretory vesicles are present These findings confirm earlier results obtained from serial sectioning of HP frozen or chemically fixed Micrasterias cells and TEM (Meindl et al., 1992) The trans-most cisterna is frequently separated from the dictyosome and appears circular (Fig 2) Depending on how it is oriented it may be assigned to a TGN Like in other plant cells (Faso et al., 2009; Moreau et al., 2007) almost all dictyosomes are in close spatial relationship to an ER cisterna at their cis-side (Figs 2, 3b, 5, 6, Suppl animation) and transitorial vesicles between these two compartments of the endomembrane system are visible For the first time FIB-serial sectioning and 3-D reconstruction shows that the dictyosomes in Micrasterias are almost entirely engulfed by a huge ER sheath which is not limited to the cis-Golgi side but also envelopes the trans-Golgi area to a large extent (Figs and 6, Suppl animation) Frequently the membranes of the trans-cisternae are in close 206 G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 Fig.3 TEM micrographs of ultrathin sections of high-pressure frozen and freeze substituted interphase cells of M denticulata (a) Dictyosomes with adjacent ER cisterna at cis- and trans-side Trans-most cisterna is chain-like constricted Large mucilage vesicles (MV) are in contact with rims of trans-cisternae Two MVBs (arrows) are located in close proximity to the trans-Golgi side and to a trans-ER cisterna (b) MVB (arrow) is in contact with vacuolar membrane translucent vesicles (arrow head) are in contact with trans-dictyosomal cisterna and MVB ER = endoplasmic reticulum (c) Representative MVB of Micrasterias with intraluminal vesicles (d) Trans-side of dictyosome (D) with stack of mucilage vesicles (MV) Three MVBs (arrows) are in close proximity to the dictyosome and to a trans-ER cisterna ER = endoplasmic reticulum (e) Dictyosome and parts of the enwrapping ER Contact between MVB (arrow) and part of a trans-ER cisterna visible MV = mucilage vesicle; ER = endoplasmic reticulum; P = Plastid (f) Part of a dictyosome and MVB attached to an ER cisterna ER = endoplasmic reticulum (g,h) MVBs in spatial contact with small electron-dense vesicle (arrow) and with larger translucent vesicle (arrow head) (i,j) MVBs attached to mucilage vesicles (MV) (j) Intraluminal vesicle of MVB discharged into upper mucilage vesicle (framed area) M = mitochondrion contact with the ER membranes either directly or via vesicular connections (Fig 6) This finding yields a new picture of the close spatial connection of the ER-Golgi machinery which became only possible by the capability of FIB/SEM tomography of providing 3-D analysis of large volumes particularly in z-direction Although single ER cisternae have been observed in vicinity to the dictyosomal trans-cisternae in TEM as well (Fig 3b), the presence of such a huge enwrapping ‘‘trans-ER’’ sheath would have been never deducible from 2-D TEM micrographs The fact that several dictyosomes of a cell can be serial sliced and visualized by FIB/SEM at a time, enables comparison of different Golgi-ER associations thus yielding additional information on the generality of these observations MVBs in Micrasterias are mostly found in close association to dictyosomes both in interphase cells (Figs and 8) and during cell growth (not shown) As in higher plant cells (Lam et al., 2007; Otegui and Spitzer, 2008; Otegui et al., 2006; Scheuring et al., 2011; Wang et al., 2011) they appear always spherical and contain intraluminal vesicles with a diameter of about 50 nm in Micrasterias (Fig 3c) Their maximum diameter averages 400 nm Several MVBs may be found in close vicinity of one dictyosome (Fig 3d) All previous studies on MVB maturation mostly done in protein storage tissue, have indicated that they originate from either the TGN or from dictyosomal derived vesicles that fuse to form a MVB (see references above) Our study employing FIB/SEM analysis provides evidence that MVB formation in Micrasterias is not only a function of the trans-Golgi region but involves a ‘‘trans-ER’’ as well Most of the MVBs investigated in Micrasterias were in spatial contact to both, an ER and a trans-dictyosomal cisterna Examples of these contacts are visible in the series of Figs and Occasionally direct contacts existed exclusively between MVB and ER although the MVB was located in close vicinity to trans-Golgi cisternae (Fig 9a,b, Suppl animation) The contact between the membranes of the ER and the MVB appears to be a direct one: membranes of ER and MVBs are frequently attached to each other (Fig 3e,f) Connections to dictyosomal derived tubular structures indicating that MVBs originate from the TGN as observed in Arabidopsis root tips G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 207 discharged into the mucilage vesicle (Fig 3j) Frequently contacts to several compartments existed simultaneously Discussion Fig.4 3-D reconstruction of interphase dictyosome of Micrasterias with enwrapping ER system (blue) and different vesicles populations Small secretory vesicles are shown in green, mucilage vesicles in grey Dictyosomal cis-side in red, transside in green Fig.5 3-D reconstruction of dictyosome and ER envelope (blue) at cis- and transside of the dictyosome Two MVBs (yellow) are visible in proximity of the dictyosomal trans-cisternae (Scheuring et al., 2011) were never found in Micrasterias Two different vesicle populations were frequently seen in contact with MVBs: small electron-dense vesicles with a diameter of approx 50 nm corresponding to the intraluminal vesicles of the MVBs both in size and in electron density and larger, electron translucent vesicles with an average diameter of 130 nm (Fig 3g,h) Electron translucent vesicles were frequently found to be in contact to the rims of trans-cisternae suggesting that they originate from the dictyosomes (Fig 3b) whereas the origin of the small vesicles is unclear Contacts between the MVBs and the dictyosomal cisternae may occur either via these vesicles, or directly between the dictyosomal membrane and the membrane of the MVB (Fig 7) Most contacts between MVBs and dictyosomes were observed with the outermost trans-cisterna or with one of the other trans-cisternae, only rarely with medium cisternae MVBs with no visible contact to either the ER or a dictyosome were also rarely found by FIB/ SEM tomography However, it cannot be excluded that the corresponding endomembrane system in these cases was located in a larger distance above or below the MVB and was simply not included in the respective series In addition to their structural connections to trans-Golgi cisternae and the ER, MVBs were observed to be in contact with each other (Figs and 9a,b) and with vacuoles (Fig 3b) Occasionally MVBs were found tightly attached to membranes of large mucilage vesicles (Fig 3i) and their transluminal vesicles seemed to be Technical advances by FIB/SEM analysis and subsequent 3-D reconstruction provides new insight into architecture of interphase dictyosomes and into formation of MVBs in the unicellular green alga Micrasterias The most important new result is the 3-D visualization of a huge ER sheath at the trans-side of the dictyosomes which together with the common cis-Golgi associated ER system known from different plant cells (among others see Hawes and Satiat-Jeunemaitre (2005), Moreau et al (2007)) almost entirely enwraps the dictyosomes in Micrasterias Neither TEM serial sectioning nor electron tomography would be able to provide information on the magnitude of this ER envelope Due to the relatively thick sections (60–70 nm) information is lost in TEM and only parts of this ‘‘trans-ER system’’ are depicted On the other hand, electron tomography is limited to a relatively small cytoplasmic volume and would not allow calculating such large cytoplasmic areas Additionally our FIB/SEM series indicate that this ‘‘trans-ER’’ sheath may also be involved in MVB formation which has been so far attributed solely to trans-Golgi compartments and their derivatives in higher plant cells (e.g (Scheuring et al., 2011; Tse et al., 2004; Wang et al., 2011)) The presence of a ‘‘trans-ER’’ system is well known from mammalian secretory cells where it represents a specialized ER cisterna in close association with the trans-most Golgi cisterna (reviewed by Mogelsvang et al (2004)) In higher plant cells indications for a ‘‘trans-ER’’ possibly involved in secretion in concert with the dictyosomes, have been obtained from early thick-sectioning techniques in mung bean cells revealing direct connections between the ER and trans-dictyosome cisternae (Harris and Oparka, 1983) However, in the recent literature referring preferentially to cryo-fixed samples or to studies in living cells, reports of the presence of a trans-Golgi-ER association are missing (see reviews by Faso et al (2009), Hawes and Satiat-Jeunemaitre (2005)) From an evolutionary point of view it is interesting that this trans-GolgiER association appears in an alga such as Micrasterias which is closely related to higher plants (Wodniok et al., 2011) Moreover, the FIB/SEM series show that direct structural contacts between the ‘‘trans-ER’’ and the trans-most Golgi cisterna – as postulated by early studies in mammalian and plant cells (Hand and Oliver, 1977; Harris and Oparka, 1983; Novikoff et al., 1971) – in fact occur in Micrasterias The presence of structural connections of MVBs not only to trans-Golgi cisternae and their derivatives but also to a ‘‘transER’’ may point towards a particular way of degradation According to the early GERL hypothesis of Novikoff et al (1971) postulating that newly synthesized lysosomal enzymes are directly delivered from the ER to the trans-most Golgi cisterna in neurons, the ER in Micrasterias may supply MVBs with lytic enzymes whereas the cargo proteins are secreted through the Golgi apparatus In this way the MVBs would become lytic compartments and starting points for degradation as postulated in early TEM studies (Tanchak and Fowke, 1987) In fact an increase in the number of MVBs has been observed in Micrasterias upon exposure to environmental stress such as high salinity or cadmium exposure (Affenzeller et al., 2009a; Andosch et al., 2012), indicating their involvement in stress induced degradation Golgi-derived vesicles resembling the ‘‘dense vesicles’’ carrying storage proteins in cotyledons or embryos of legumes (Hinz et al., 1999; Otegui and Spitzer, 2008; Robinson et al., 1998) and electron-dense small vesicles with the same size as the interluminal vesicles have been found to be in contact with MVBs in Micrasterias and are interpreted to contribute 208 G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 Fig.6 FIB/SEM series of dictyosome in contact to a cis- and a trans-ER cisterna Trans-ER covers the trans-side of the dictyosome almost entirely At least two of the transcisternae (framed areas) are in contact with the trans-ER either directly or via vesicular connections The trans-most cisterna is vesicular and disconnected from Golgi stack appearing as TGN Large mucilage vesicles (MV) are visible in close vicinity to dictyosome 10 nm slices, every 10th image shown to their formation Our data on frequent, close structural contacts between different compartments suggest that discharge of MVBs occurs both into vacuoles or lytic compartments but also into mucilage vesicles Mucilage vesicles are secreted throughout the cell cycle of Micrasterias (Oertel et al., 2004) and were recently found to represent vehicles for heavy metal detoxification (Volland G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 209 Fig.7 FIB/SEM series of MVB in contact with trans-most dictyosomal cisterna via small vesicles (arrow) Maturating and ripe mucilage vesicle in contact to each other and close to trans-Golgi cisternae 10 nm slices, every 4th image shown Fig.8 FIB/SEM series of MVB in direct spatial contact to both a trans-dictyosomal cisterna and a trans-ER cisterna (arrow) The MVB also contacts one of the maturating mucilage vesicles et al., 2011) Heavy metals are sequestered in mucilage vesicles and removed from the cell by mucilage secretion In the same way degrading proteins inside MVBs may be disposed via the secretion pathway Cytochemical and immuno-TEM studies including cells after stress exposure will be required to verify this hypothesis 210 G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 Fig.9 (a,b) 3-D reconstruction of spatial relationship between trans-Golgi cisternae and MVBs (yellow) without (a) and with (b) enwrapping ER system (blue) The reconstructions show that the membranes of the MVBs are in direct contact with the membranes of the ER but not with the Golgi cisternae Acknowledgments We gratefully acknowledge the excellent technical assistance by Silvia Dobler and Ancuela Andosch and the valuable suggestions and support by Max Scheungrab during the manual segmentation for the 3-D reconstructions The study was financially supported by the Austrian Science Fund project 21035-B16 to U.L-M Appendix A Supplementary data Supplementary data associated with this article can be found, in the online version, at http://dx.doi.org/10.1016/j.jsb.2013.10.003 References Affenzeller, M.J., Darehshouri, A., Andosch, A., Lütz, C., Lütz-Meindl, U., 2009a Salt stress-induced cell death in the unicellular green alga Micrasterias denticulata J Exp Bot 60, 939–954 Affenzeller, M.J., Darehshouri, A., Andosch, A., Lütz, C., Lütz-Meindl, U., 2009b PCD and autophagy in the unicellular green alga Micrasterias denticulata Autophagy 5, 854–855 Aichinger, N., Lütz-Meindl, U., 2005 Organelle interactions and possible degradation pathways visualized in high-pressure frozen algal cells J Microsc 219, 86–94 Andosch, A., Affenzeller, M.J., Lütz, C., Lütz-Meindl, U., 2012 A freshwater green alga under cadmium stress: ameliorating calcium effects on ultrastructure and photosynthesis in the unicellular model Micrasterias J Plant Physiol 169, 1489–1500 Bassham, D.C., Laporte, M., Marty, F., Moriyasu, Y., Ohsumi, Y., Olsen, L.J., Yoshimoto, K., 2006 Autophagy in development and stress responses of plants Autophagy 2, 2–11 Darehshouri, A., Affenzeller, M., Lütz-Meindl, U., 2008 Cell death upon H2O2 induction in the unicellular green alga Micrasterias Plant Biol 10, 732–745 Donohoe, B.S., Mogelsvang, S., Staehelin, L.A., 2006 Electron tomography of ER, Golgi and related membrane systems Methods 39, 154–162 Eder, M., Lütz-Meindl, U., 2008 Pectin-like carbohydrates in the green alga Micrasterias characterized by cytochemical analysis and energy filtering TEM J Microsc 231, 201–214 Eder, M., Tenhaken, R., Driouich, A., Lütz-Meindl, U., 2008 Occurrence and characterization of arabinogalactan-like proteins and hemicelluloses in Micrasterias (Streptophyta) J Phycol 44, 1221–1234 Faso, C., Boulaflous, A., Brandizzi, F., 2009 The plant Golgi apparatus: last 10 years of answered and open questions FEBS Lett 583, 3752–3757 Hand, A.R., Oliver, C., 1977 Relationship between Golgi apparatus, Gerl, and secretory granules in acinar cells of rat exorbital lacrimal gland J Cell Biol 74, 399–413 Harris, N., Oparka, K.J., 1983 Connections between dictyosomes, ER and GERL in cotyledons of mung bean (Vigna radiata L.) Protoplasma 114, 93–102 Hawes, C., 2005 Cell biology of the plant Golgi apparatus New Phytol 165, 29–44 Hawes, C., Satiat-Jeunemaitre, B., 2005 The plant Golgi apparatus-going with the flow Biochim Biophys Acta 1744, 466–480 Hayashi-Nishino, M., Fujita, N., Noda, T., Yamaguchi, A., Yoshimori, T., Yamamoto, A., 2009 A subdomain of the endoplasmic reticulum forms a cradle for autophagosome formation Nat Cell Biol 11, 1433–1437 Hinz, G., Hillmer, S., Bäumer, M., Hohl, I.I., 1999 Vacuolar storage proteins and the putative vacuolar sorting receptor BP-80 exit the Golgi apparatus of developing pea cotyledons in different transport vesicles Plant Cell 11, 1509–1524 Hwang, I., Robinson, D.G., 2009 Transport vesicle formation in plant cells Curr Opin Plant Biol 12, 660–669 Kang, B.H., Staehelin, L.A., 2008 ER-to-Golgi transport by COPII vesicles in Arabidopsis involves a ribosome-excluding scaffold that is transferred with the vesicles to the Golgi matrix Protoplasma 234, 51–64 Kang, B.H., Nielsen, E., Preuss, M.L., Mastronarde, D., Staehelin, L.A., 2011 Electron tomography of RabA4b- and PI-4Kbeta1-labeled trans Golgi network compartments in Arabidopsis Traffic 12, 313–329 Knott, G., Marchman, H., Wall, D., Lich, B., 2008 Serial section scanning electron microscopy of adult brain tissue using focused ion beam milling J Neurosci 28, 2959–2964 Lam, S.K., Siu, C.L., Hillmer, S., Jang, S., An, G.H., Robinson, D.G., Jiang, L.W., 2007 Rice SCAMP1 defines clathrin-coated, trans-Golgi-located tubular-vesicular structures as an early endosome in tobacco BY-2 cells Plant Cell 19, 296–319 Lehner, C., Kerschbaum, H.H., Lütz-Meindl, U., 2009 Nitric oxide suppresses growth and development in the unicellular green alga Micrasterias denticulata J Plant Physiol 166, 117–127 Lütz-Meindl, U., Brosch-Salomon, S., 2000 Cell wall secretion in the green alga Micrasterias J Microsc 198, 208–217 Lütz-Meindl, U., Aichinger, N., 2004 Use of energy-filtering transmission electron microscopy for routine ultrastructural analysis of high-pressure-frozen or chemically fixed plant cells Protoplasma 223, 155–162 Marty, F., 1978 Cytochemical studies on GERL, provacuoles, and vacuoles in root meristematic cells of Euphorbia Proc Natl Acad Sci U.S.A 75, 852–856 Marty, F., 1999 Plant vacuoles Plant Cell 11, 587–600 Meindl, U., 1993 Micrasterias cells as a model system for research on morphogenesis Microbiol Rev 57, 415–433 Meindl, U., Lancelle, S., Hepler, P., 1992 Vesicle production and fusion during lobe formation in Micrasterias visualized by high-pressure freeze fixation Protoplasma 170, 104–114 Mogelsvang, S., Marsh, B.J., Ladinsky, M.S., Howell, K.E., 2004 Predicting function from structure: 3D structure studies of the mammalian Golgi complex Traffic 5, 338–345 Moreau, P., Brandizzi, F., Hanton, S., Chatre, L., Melser, S., Hawes, C., SatiatJeunemaitre, B., 2007 The plant ER-Golgi interface: a highly structured and dynamic membrane complex J Exp Bot 58, 49–64 Novikoff, P.M., Novikoff, A.B., Quintana, N., Hauw, J.J., 1971 Golgi apparatus, GERL, and lysosomes of neurons in rat dorsal root ganglia, studied by thick section and thin section cytochemistry J Cell Biol 50, 859–886 Oertel, A., Aichinger, N., Hochreiter, R., Thalhamer, J., Lütz-Meindl, U., 2004 Analysis of mucilage secretion and excretion in Micrasterias (Chlorophyta) by means of immune electron microscopy and digital time lapse video microscopy J Phycol 40, 711–720 Otegui, M.S., Spitzer, C., 2008 Endosomal functions in plants Traffic 9, 1589–1598 Otegui, M.S., Herder, R., Schulze, J., Jung, R., Staehelin, L.A., 2006 The proteolytic processing of seed storage proteins in Arabidopsis embryo cells starts in the multivesicular bodies Plant Cell 18, 2567–2581 Robinson, D.G., Jiang, L., Schumacher, K., 2008 The endosomal system of plants: charting new and familiar territories Plant Physiol 147, 1482–1492 Robinson, D.G., Bäumer, M., Hinz, G., Hohl, I., 1998 Vesicle transfer of storage proteins to the vacuole: the role of the Golgi apparatus and multivesicular bodies J Plant Physiol 152, 659–667 Salomon, S., Meindl, U., 1996 Brefeldin A induces reversible dissociation of the Golgi apparatus in the green alga Micrasterias Protoplasma 194, 231– 242 Scheuring, D., Viotti, C., Krüger, F., Künzl, F., Sturm, S., Bubeck, J., Hillmer, S., Frigerio, L., Robinson, D.G., Pimpl, P., Schumacher, K., 2011 Multivesicular bodies mature from the trans-Golgi network/early endosome in Arabidopsis Plant Cell 23, 3463–3481 Schlösser, U.G., 1982 Sammlungen von Algenkulturen Ber Deutsch Bot Ges 95, 181–276 Schroeder-Reiter, E., Wanner, G., 2009 Chromosome centromeres: structural and analytical investigations with high resolution scanning electron microscopy in combination with focused ion beam milling Cytogenet Genome Res 124, 239– 250 Schroeder-Reiter, E., Perez-Willard, F., Zeile, U., Wanner, G., 2009 Focused ion beam (FIB) combined with high resolution scanning electron microscopy: a promising tool for 3D analysis of chromosome architecture J Struct Biol 165, 97–106 Schroeder-Reiter, E., Sanei, M., Houben, A., Wanner, G., 2012 Current SEM techniques for de- and re-construction of centromeres to determine 3D CENH3 distribution in barley mitotic chromosomes J Microsc 246, 96–106 G Wanner et al / Journal of Structural Biology 184 (2013) 203–211 Staehelin, L.A., Moore, I., 1995 The plant Golgi-apparatus – structure, functionalorganization and trafficking mechanisms Annu Rev Plant Physiol Plant Mol Biol 46, 261–288 Staehelin, L.A., Giddings Jr., T.H., Kiss, J.Z., Sack, F.D., 1990 Macromolecular differentiation of Golgi stacks in root tips of Arabidopsis and Nicotiana seedlings as visualized in high pressure frozen and freeze-substituted samples Protoplasma 157, 75–91 Tanchak, M.A., Fowke, L.C., 1987 The morphology of multivesicular bodies in soybean protoplasts and their role in endocytosis Protoplasma 138, 173–182 Tse, Y.C., Mo, B., Hillmer, S., Zhao, M., Lo, S.W., Robinson, D.G., Jiang, L., 2004 Identification of multivesicular bodies as prevacuolar compartments in Nicotiana tabacum BY-2 cells Plant Cell 16, 672–693 Villinger, C., Gregorius, H., Kranz, C., Höhn, K., Münzberg, C., von Wichert, G., Mizaikoff, B., Wanner, G., Walther, P., 2012 FIB/SEM tomography with TEM-like resolution for 3D imaging of high-pressure frozen cells Histochem Cell Biol 138, 549–556 Viotti, C., Bubeck, J., Stierhof, Y.D., Krebs, M., Langhans, M., van den Berg, W., van Dongen, W., Richter, S., Geldner, N., Takano, J., Jürgens, G., de Vries, S.C., 211 Robinson, Schumacher, K., 2010 Endocytic and secretory traffic in Arabidopsis merge in the trans-Golgi network/early endosome, an independent and highly dynamic organelle Plant Cell 22, 1344–1357 Volland, S., Andosch, A., Milla, M., Stöger, B., Lütz, C., Lütz-Meindl, U., 2011 Intracellular metal compartmentalization in the green algal model system Micrasterias denticulata (Streptophyta) measured by transmission electron microscopy–coupled electron energy loss spectroscopy J Phycol 47, 565–579 Wang, J., Tse, Y.C., Hinz, G., Robinson, D.G., Jiang, L., 2011 Storage globulins pass through the Golgi apparatus and multivesicular bodies in the absence of dense vesicle formation during early stages of cotyledon development in mung bean J Exp Bot 63, 1367–1380 Wodniok, S., Brinkmann, H., Glöckner, G., Heidel, A.J., Philippe, H., Melkonian, M., Becker, B., 2011 Origin of land plants: conjugating green algae hold the key? BMC Evol Biol 11, 104 Ylä-Anttila, P., Vihinen, H., Jokitalo, E., Eskelinen, E.L., 2009 3D tomography reveals connections between the phagophore and endoplasmic reticulum Autophagy 5, 1180–1185