It is still unclear why some proteins that travel along the secretory pathway are retained in the Golgi complex whereas others make their way to the plasma membrane. Recent bioinformatic analyses on a large number of single-spanning membrane proteins support the hypothesis that specific features of the transmembrane domain (TMD) are relevant to the sorting of these proteins to particular organelles. Here we experimentally test this hypothesis for Golgi and plasma membrane proteins. Using the Golgi SNARE protein Sft1 and the plasma membrane SNARE protein Sso1 from Saccharomyces cerevisiae as model proteins, we modified the length of their TMDs and the volume of their exoplasmic hemi-TMD, and determined their subcellular localization both in yeast and mammalian cells. We found that short TMDs with high-volume exoplasmic hemi-TMDs confer Golgi membrane residence, whereas TMDs with low-volume exoplasmic hemi-TMDs, either short or long, confer plasma membrane residence to these proteins. Results indicate that the shape of the exoplasmic hemi-TMD, in addition to the length of the entire TMD, determine retention in the Golgi or exit to the plasma membrane of Type II membrane proteins.
Proteins of the secretory pathway are transported by tubulo-vesicular carriers from their site of synthesis in the endoplasmic reticulum (ER) to the plasma membrane and the cell exterior. It is still an open question why Golgi-resident proteins concentrate in this organelle whereas other proteins do not, following the route towards the plasma membrane instead. For 16 yeast glycosyltransferases an FLxK amino acid motif in the cytoplasmic tail determines Golgi retention through interaction with the COPI-interacting protein Vps74 (Tu et al., 2008). Other reports assign importance to the TMD for localization of glycosyltransferases (GTs) in the Golgi (Opat et al., 2001; Tang et al., 1992; Teasdale et al., 1992). This capacity was attributed to particular amino acid residues in the TMD (Aoki et al., 1992; Sousa et al., 2003) or the length of the TMD (Bretscher and Munro, 1993; Rayner and Pelham, 1997; Ronchi et al., 2008). Recent analyses of a large protein dataset showed that TMDs from single-spanning membrane proteins of the Golgi and plasma membrane have distinctive geometric features: Golgi protein TMDs are on average four amino acid residues shorter than those of plasma membrane proteins in vertebrates, and seven residues shorter in fungi. Also, they have a higher concentration of amino acid residues with high-volume side chains in the exoplasmic hemi-TMD (Sharpe et al., 2010). Previous experimental evidence of these TMD features as determinants of organelle residence only addressed the effect of TMD length (Munro, 1995; Ronchi et al., 2008). Here we tested whether both length and volume of TMDs are bona fide determinants for localization of Type II membrane proteins in the Golgi complex or the plasma membrane. The S. cerevisiae SNARE (soluble NSF attachment protein receptor) proteins Sft1 and Sso1, whose TMDs display representative geometric features of Golgi and plasma membrane proteins, respectively, were selected as model proteins. We show that modifying the length of the TMDs of these proteins or the volume of their exoplasmic hemi-TMDs, dramatically affects their subcellular localization, demonstrating that both features are major determinants for retention in the Golgi or exit to the plasma membrane.
Results and Discussion
Bioinformatic analyses reveals differences in length and shape of TMDs between Golgi and plasma membrane type II membrane proteins
The results of the analysis of our dataset (supplementary material Table S1), which consists of 472 Golgi and 395 pm type II metazoan membrane proteins, are shown in Fig. 1A. A plot of mean hydrophobicity for each TMD position of proteins in the dataset showed similar average hydrophobicity values for the hydrophobic core of plasma membrane and Golgi proteins. However, the length of the core was longer for plasma membrane proteins (supplementary material Fig. S1). TMD lengths of Golgi proteins (of which 79% are putative glycosyltransferases) had a median value of 18 aa (18.2±2.9; mean ± s.d.) and residues of the exoplasmic hemi-TMD had an average volume of 150.9 Å3. TMD lengths of plasma membrane proteins had a median of 22 aa (21.1±3.8; mean ± s.d.) and residues of the exoplasmic hemi-TMD had an average volume of 139.6 Å3. These results agree with a previous study (Sharpe et al., 2010). In Fig. 1B, the volume of the first seven amino acids of the exoplasmic hemi-TMD is plotted against TMD length for each protein in the dataset. Most Golgi proteins (74%) in the dataset were included in a region delimited by maximum TMD length of 21 amino acids and minimum average exoplasmic hemi-TMD volume of 134 Å3, which excludes most (75%) plasma membrane proteins.
Analysis of the amino acid composition of Golgi and plasma membrane TMDs revealed similarities in their cytoplasmic hemi-TMDs but significant differences in their exoplasmic hemi-TMDs: Golgi proteins displayed increased numbers of aromatic amino acids (particularly tyrosine, Y), whereas plasma membrane proteins display increased amounts of the small amino acids Ala and Gly (supplementary material Table S2). About 65% of Golgi protein exoplasmic hemi-TMDs had two or more aromatic, high-volume amino acids (Tyr, Phe, Trp), whereas 60% of plasma membrane protein exoplasmic hemi-TMDs had none or one (Fig. 1C). Additionally, 75% of Golgi proteins contained none or one small amino acid (Ala or Gly), whereas 65% of plasma membrane proteins had two or more (Fig. 1D). Both Golgi and plasma membrane proteins had diminished amounts of Leu and Ile in their exoplasmic hemi-TMDs.
TMD features determine Golgi or plasma membrane localization
We experimentally tested whether TMD features determine Golgi or plasma membrane localization using wild-type or specific chimeric yeast SNARE proteins that differ only in a few residues of their TMDs and display robust localization phenotypes. Sft1 is a Golgi protein with a short TMD (16 aa) and high-volume residues in its exoplasmic hemi-TMD. Sso1 is a plasma membrane protein with a longer TMD (22 aa) and with less-voluminous residues at its exoplasmic hemi-TMD (Fig. 1B and Fig. 2). The Sso1 TMD is sufficient for plasma membrane localization (Rayner and Pelham, 1997) and its cytoplasmic domain lacks endocytic signals (Valdez-Taubas and Pelham, 2003). Sft1 and Sso1 show a well-defined subcellular distribution in yeast even when overexpressed (Aalto et al., 1993; Banfield et al., 1995). Myc-tagged versions of the wild-type SNARE proteins or their chimeric variants (Fig. 2) were transformed into yeast and their subcellular localization was established by immunofluorescence (Fig. 3). Substituting the whole TMD of Sft1 for that of Sso1 [Sft1(Sso1)], resulted in a clear change of localization of Sft1 from the Golgi to the plasma membrane (Fig. 3A,B) and vice versa: substituting the Sso1 TMD for that of Sft1 [Sso1(Sft1)] led to Golgi localization of Sso1 (Fig. 3C,D). Colocalization experiments with the late-Golgi marker Chc1 confirmed the Golgi localization of the observed intracellular punctate structures (supplementary material Fig. S2). Results indicate that the TMDs of Sft1 and Sso1 act as determinants for Golgi and plasma membrane localization, respectively.
Exoplasmic hemi-TMD volume is a subcellular localization determinant
We next examined whether determinants of subcellular localization were present in the exoplasmic or the cytoplasmic hemi-TMDs. Sft1 with the cytoplasmic hemi-TMD of Sso1 [Sft1(Sso18-Sft18)], remained in the Golgi complex (Fig. 3E), but localized at the plasma membrane when its exoplasmic hemi-TMD was substituted by the less voluminous, albeit shortened, version of the exoplasmic half of Sso1 [Sft1(Sft18-Sso18)] (Fig. 3G). Sft1 with the whole Sso1 exoplasmic hemi-TMD and an extended cytoplasmic Sft1 hemi-TMD [Sft1(Sft111-Sso111)] also localized to the plasma membrane (Fig. 3H). Noticeably, a long TMD with the cytoplasmic half of Sso1 and an extended exoplasmic half of Sft1 [Sft1(Sso111-Sft111)] left the Golgi and localized at the plasma membrane (Fig. 3F). Constructs bearing the cytoplasmic domain of Sso1, gave essentially the same results: a short TMD with a high-volume exoplasmic hemi-TMD caused Golgi retention of Sso1 [Sso1(Sso18-Sft18)] (Fig. 3I); and either a short TMD with less-voluminous exoplasmic hemi-TMD [Sso1(Sft18-Sso18] (Fig. 3K) or longer TMDs of any volume, Sso1(Sso111-Sft111) and Sso1(Sft111-Sso111), resulted in plasma membrane localization of the chimeras (Fig. 3H,J). The idea that the presence of an amino acid motif in the exoplasmic hemi-TMD of Sft1 acts as a specific Golgi-retention signal was discarded because a construct with scrambled residues in this region [Sso1(Sso18-Sft18scr)] (Fig. 2) still localized to the Golgi (Fig. 3M).
These experiments indicate that both short length and a high-volume exoplasmic hemi-TMD are crucial parameters to confer Golgi localization to the chimeras because replacement of Sft1 exoplasmic hemi-TMD with less-voluminous amino acid residues or extension of the exoplasmic hemi-TMD with residues of any volume results in localization at the plasma membrane.
Features of the exoplasmic hemi-TMDs define Golgi or plasma membrane localization in mammalian cells
To examine whether the geometric features of TMDs also act as determinants of localization in mammalian cells, CHO-K1 cells were transfected with mCherry-tagged Sso1 or fusions of the Sso1 cytoplasmic domain to the TMDs described in Fig. 2 and their subcellular localization was established by colocalization with the plasma membrane marker K-Ras (Gomez and Daniotti, 2005), the Golgi complex marker GalT2 or the trans-Golgi network marker GalNAcT (Giraudo et al., 2001), all of which were tagged with YFP. Wild-type Sso1 colocalized with K-Ras, but when its TMD was replaced with that of Sft1, it colocalized partially with GalT2 and to a greater extent with GalNAcT (Fig. 4A). Longer TMDs, Sso1(Sso111-Sft111) and Sso1(Sft111-Sso111), resulted in plasma membrane localization of Sso1 whereas a short TMD with a high-volume exoplasmic hemi-TMD, Sso1(Sso18-Sft18), resulted in Golgi localization. Unexpectedly, the chimera with short and less-voluminous exoplasmic hemi-TMD [Sso1(Sft18-Sso18] localized to mitochondria, where it colocalized with the Mitotracker marker (supplementary material Fig. S3A). The ratio of fluorescence of Sso1 in the Golgi or trans-Golgi network to that in the plasma membrane increased five- to ten-fold, respectively, when its TMD was either substituted for the whole Sft1 TMD [Sso1(Sft1)], or when just the exoplasmic hemi-TMD was substituted for that of Sft1 [Sso1(Sso18-Sft18)] (Fig. 4B). Chimeras bearing long TMDs, Sso1(Sso111-Sft111) and Sso1(Sft111-Sso111), displayed values comparable to that of wild-type Sso1 (Fig. 4B). It was verified that wild-type Sso1 traffics through the Golgi because it localized to the Golgi when exit was blocked at 20°C (supplementary material Fig. S3B). Therefore, results in S. cerevisiae are essentially reproduced in mammalian cells. Similar trends were found in the Arabidopsis membrane proteome (Nikolovski et al., 2012), suggesting that these TMDs features are indeed widespread determinants of Golgi or plasma membrane residence.
The results presented here highlight the relevance of the volume of the exoplasmic hemi-TMD, which might add to the geometric mismatch imposed by the length in determining Golgi or plasma membrane residence. An appealingly simple hypothesis is that the more voluminous exoplasmic hemi-TMDs of Golgi proteins negatively affect their fit into the highly curved membrane domains from which Golgi transport carriers enriched in cholesterol and sphingolipids originate (Duran et al., 2012; Klemm et al., 2009; Polishchuk et al., 2003). By contrast, TMDs from plasma membrane proteins could conform a complex, thermodynamically favourable association with these order-inducing lipids and exit the Golgi.
Large exoplasmic amino acid residues could also discourage Golgi proteins from loading into the curved membranes of COPI vesicles. However, these membranes are poor in order-inducing lipids (Klemm et al., 2009), and might accommodate voluminous exoplasmic hemi-TMDs, allowing Golgi proteins to be loaded into COPI vesicles. Interactions of cytoplasmic tail amino acid motifs such as FLxK in yeast with the COPI-coat-interacting VPS74 protein (Tu et al., 2008), might also promote loading into these vesicles. However, this motif was infrequent in Golgi proteins of our dataset (Maccioni et al., 2011).
Finally, interactions with unidentified cargo receptors that could recognize TMDs by their length and exoplasmic volume, similar to what has been described for the ER cargo receptor Erv14 (Herzig et al., 2012), could also lead to loading of Golgi proteins into COPI vesicles.
Materials and Methods
Plasmids and strains
Yeast (SEY6210) expression experiments were performed using pRS316-based plasmids containing the TPI1 promoter, the Myc tag, wild-type or chimeric SNARE proteins and the PEP12 terminator. A plasmid bearing a fusion of Sft1t to the Sso1 TMD (pJV481) was used in in vivo gap repair experiments to generate all chimeric TMD constructs. DNA fragments encoding synthetic transmembrane domains and regions of homology to pJV481 were ordered from Genscript. A HindIII site in SSO1 was removed and this fragment was used to replace the Sft1 cytoplasmic domain in the plasmids described above. Golgi colocalization experiments in yeast were performed on the LCY1389 strain (kindly provided by Elizabeth Conibear), in which genomically encoded Chc1 (clathrin heavy-chain) was C-terminally tagged with RFP. Mammalian expression vectors were generated by introducing wild-type and chimeric SNARE proteins in pmCherry-C1 (Clontech). All plasmids were verified by DNA sequencing. Western blot analyses for both yeast and mammalian cells indicated that all chimeras displayed the expected electrophoretic mobility and expression levels comparable to those of the wild-type proteins (supplementary material Fig. S4).
193 human proteins with annotated subcellular location and Type II transmembrane topology were gathered from the SwissProt database. 2796 metazoan orthologs were gathered from the ORTHOMCL database; redundancy was reduced using CD-HIT to cluster sequences with more than 70% sequence identity; 842 Golgi proteins and 439 plasma membrane proteins were subjected to confirmation of Type II topology, carried out by TMD prediction using HMMTOP with constrained predictions (N-terminus cytoplasmic, C-terminus extracytoplasmic). A 12-amino-acid sliding window analysis, using the GES scale (Engelman et al., 1986), was used to identify the hydrophobic core of the TMDs. Positions of the edges of the hydrophobic core were used as starting points for an analysis using a hydropathy window of five amino acids with the GES scale, and a cut-off of −0.4 to scan for TMD edges (PERL scripts written in our laboratory). When the sliding window average detected a TMD edge with a charged amino acid, the edge was moved one residue towards the core. Proteins for which a TMD edge could not be effectively determined were removed from the dataset. Amino acid volume analysis was performed with the volume scale TSAJ990102 (Tsai et al., 1999) from AA index, using PERL scripts written in the laboratory on the final dataset, which consists of 472 Golgi proteins and 397 plasma membrane type II membrane proteins.
Immunofluorescence and microscopy
Exponentially growing yeast cells were fixed, spheroplasted, permeabilized and treated with anti Myc monoclonal antibody (Sigma). Mammalian and yeast cells were observed in an Olympus FluoView FV1000 confocal microscope.
Fluorescence intensity quantification in CHO-K1 cells
Image processing was performed using ImageJ software (NIH, Bethesda, MD; http://rsb.info.nih.gov/ij/). Using the YFP channel, a threshold was applied to differentiate pixels corresponding to the particular organelle, and a binary mask was created. Fluorescence images of chimeric proteins were obtained by multiplication of this binary mask with the background-subtracted image of the mCherry channel. For each organelle marker, the ratio of integrated fluorescence intensity in this region relative to the integrated fluorescence intensity in the whole cell was calculated.
We thank B.L. Caputto, J.L. Daniotti and A.O. Cáceres for critical reading of the manuscript.
↵‡ Present address: Instituto Multidisciplinario de Biología Vegetal IMBIV (UNC-CONICET), Facultad de Ciencias Exactas y Naturales, Universidad Nacional de Córdoba, Argentina
H.J.M. and J.V.T. designed and supervised the entire project and wrote the manuscript. R.Q. conducted the bioinformatics analyses, performed experiments, and wrote the manuscript. A.T. performed experiments in yeast and mammalian cells. A.G.M. assisted with bioinformatics and performed image quantification.
This work was supported in part by Grant PICT·2566 and SECYT UNC 601 to H.J.F.M. and PICT 01102 and SECYT UNC to J.V.T. R.Q., A.G.M. and A.T. are recipients of CONICET Fellowships; H.J.F.M. and J.V.T. are Career Investigators of CONICET (Argentina).
Supplementary material available online at http://jcs.biologists.org/lookup/suppl/doi:10.1242/jcs.130658/-/DC1
- Accepted September 23, 2013.
- © 2013. Published by The Company of Biologists Ltd