Department of Biology, University of Utah, Salt Lake City, Utah 84112
In Saccharomyces cerevisiae, the growing
bud inherits a portion of the mitochondrial network
from the mother cell soon after it emerges. Although
this polarized transport of mitochondria is thought to
require functions of the cytoskeleton, there are conflicting reports concerning the nature of the cytoskeletal element involved. Here we report the isolation of a
yeast mutant, mdm20, in which both mitochondrial inheritance and actin cables (bundles of actin filaments)
are disrupted. The MDM20 gene encodes a 93-kD
polypeptide with no homology to other characterized
proteins. Extra copies of TPM1, a gene encoding the
actin filament-binding protein tropomyosin, suppress
mitochondrial inheritance defects and partially restore
actin cables in mdm20 cells. Synthetic lethality is also
observed between mdm20 and tpm1 mutant strains. Overexpression of a second yeast tropomyosin, Tpm2p,
rescues mutant phenotypes in the mdm20 strain to a
lesser extent. Together, these results provide compelling evidence that mitochondrial inheritance in yeast is
an actin-mediated process. MDM20 and TPM1 also exhibit the same pattern of genetic interactions; mutations in MDM20 are synthetically lethal with mutations
in BEM2 and MYO2 but not SAC6. Although MDM20
and TPM1 are both required for the formation and/or stabilization of actin cables, mutations in these genes
disrupt mitochondrial inheritance and nuclear segregation to different extents. Thus, Mdm20p and Tpm1p
may act in vivo to establish molecular and functional
heterogeneity of the actin cytoskeleton.
Mitochondria are essential organelles whose morphology, copy number, and distribution can vary
dramatically in different eukaryotic cell types
(Bereiter-Hahn, 1990 In the budding yeast Saccharomyces cerevisiae, respiring
mitochondria form an elaborate network of tubular membranes located near the cell periphery (Hoffman and
Avers, 1973
Most forms of organelle motility are directed by cytoskeletal structures and their associated motor proteins.
Mitochondria have been reported to colocalize with actin
filaments (Drubin et al., 1993 Recent studies have also established a role for the yeast
actin cytoskeleton in mitochondrial distribution and inheritance. Yeast cells contain a single, essential, conventional
actin gene (ACT1) (Shortle et al., 1982 To learn more about molecules that control mitochondrial inheritance, we screened a collection of yeast mutants for strains that failed to transport mitochondria into
growing buds. In one of these mutants, mdm20, both mitochondrial inheritance and the organization of actin cables
were disrupted. The MDM20 gene encodes a novel 93-kD
protein with no sequence similarities to proteins in the
database. Extra copies of TPM1, a gene encoding the actin filament-binding protein tropomyosin, partially restored
actin cables and suppressed mitochondrial inheritance defects in the mdm20 strain. Furthermore, the combination
of null mutations in MDM20 and TPM1 resulted in synthetic lethality. Overexpression of a second yeast tropomyosin, Tpm2p, also rescued actin organization defects
and mitochondrial inheritance defects in mdm20 cells, but
to a lesser extent. Together, these results provide compelling evidence that mitochondrial inheritance in yeast is an
actin-mediated process. Like tpm1, mdm20 mutations are
synthetically lethal with mutations in BEM2 (Rho-GAP)
and MYO2 (type V myosin) but not SAC6 (fimbrin). Thus,
TPM1 and MDM20 exhibit the same pattern of genetic interactions. Despite the fact that mutations in MDM20 and
TPM1 both result in the loss of observable actin cables in
cells, we found that mitochondrial inheritance and nuclear
segregation were disrupted to different extents in mdm20
and tpm1 mutant strains. Our results suggest that these
two proteins act in vivo to establish molecular and functional heterogeneity of the actin cytoskeleton.
Strains, Media, and Genetic Techniques
Yeast strains used in this study are listed in Table I. Rich medium (yeast/
peptone/dextrose [YPD] and yeast/peptone/glycerol [YPG]), synthetic medium (synthetic dextrose [SD] and synthetic galactose [SGal]), and media
containing 5-fluoro-orotic acid (5-FOA)1 were prepared as described by
Sherman et al. (1986) Table I.
Yeast Strains Used in This Study
; Yaffe, 1991
; Thorsness, 1992
; Bereiter-Hahn and Voth, 1994
; Warren and Wickner, 1996
).
Like all organelles that cannot be synthesized de novo, the
mitochondrial compartment must grow, divide, and be delivered to newly formed daughter cells during division.
While substantial progress has been made in identifying the
molecular components that mediate mitochondrial biogenesis (Hannavy et al., 1993
; Schwarz and Neupert, 1994
;
Kubrich et al., 1995
; Ryan and Jensen, 1995
; Lill and Neupert, 1996
), a detailed picture of the mechanisms that control mitochondrial morphology, distribution, and motility
throughout the cell cycle has not yet emerged.
). Very early in the cell cycle (early S phase), a
portion of this mitochondrial network is transported from
the mother cell into the growing bud (Fig. 1) (Stevens,
1981
). Recent genetic studies have identified a few proteins that control mitochondrial morphology and distribution in cells and mitochondrial transmission during cell division. These include Mdm10p and Mmm1p, two proteins
of the outer mitochondrial membrane required for the
maintenance of normal organelle morphology (Sogo and
Yaffe, 1994
, mdm [mitochondrial distribution and morphology]; Burgess et al., 1994
, mmm [maintenance of mitochondrial morphology]; Mdm2p/Ole1p, a fatty acid desaturase that may regulate the level of unsaturated fatty
acids in the mitochondrial membrane (Stukey et al., 1989
,
1990
; Stewart and Yaffe, 1991
, ole [oleic acid requiring]); and Mdm1p, a protein with characteristics of the mammalian intermediate filament-like proteins keratin and vimentin (McConnell and Yaffe, 1992
, 1993
). In addition, there
are several proteins that are required for the normal maintenance or segregation of mitochondrial DNA. Mgm1p is
a member of the dynamin family of GTP binding proteins (Jones and Fangman, 1992
; Guan et al., 1993
; Backer,
1995
; mgm [mitochondrial genome maintenance]); ILV5
encodes a protein that plays an as yet unidentified role in
mitochondrial genome maintenance (Zelenaya-Troitskaya
et al., 1995
; ilv [isoleucine-plus-valine requiring]); and Abf2p
is an HMG1-like DNA binding protein (Diffley and Stillman, 1991
, 1992
; abf [ARS binding factor]). Studies are in
progress in a number of laboratories to determine how the
activities of these proteins control the behavior of the mitochondrial compartment and the replication and segregation of the mitochondrial genome.
Fig. 1.
Mitochondrial inheritance during mitotic cell division.
Mitochondria are localized near the cortex of unbudded and budding cells. Early in the cell cycle (S phase) a portion of the maternal mitochondrial network extends into the developing bud. As
the bud grows (S phase to G2 phase), mitochondria continue to
accumulate in the daughter cell. At cytokinesis (M phase/G1 phase
boundary), the mitochondrial content of the daughter cell is often
greater than that of the mother cell.
[View Larger Version of this Image (16K GIF file)]
), microtubules (Heggeness et
al., 1978
; Ball and Singer, 1982
; Summerhayes et al., 1983
),
and intermediate filaments (Mose-Larsen et al., 1982
;
Summerhayes et al., 1983
; Stromer and Bendayan, 1990
)
in different cell types, and recent studies indicate that mitochondria can be transported in a polarized fashion using both microtubule- (Nangaku et al., 1994
; Morris and Hollenbeck, 1995
; Hollenbeck, 1996
) and actin-based (Kuznetsov et al., 1992
; Morris and Hollenbeck, 1995
; Simon et
al., 1995
; Hollenbeck, 1996
) motors. In yeast, two different
cytoskeletal elements, Mdm1p and actin, have been proposed to direct the transfer of mitochondria into yeast buds.
Mdm1p shares structural features with mammalian intermediate filament proteins and will form 10-nm filaments
in vitro (McConnell and Yaffe, 1992
, 1993
). Mutations in
MDM1 cause defects in mitochondrial morphology and
also in both mitochondrial and nuclear inheritance, suggesting that this protein is important for organelle positioning and/or segregation.
; Welch et al., 1994
).
In vivo, actin is organized into two different types of structures: (a) cortical actin patches (invaginations of the plasma
membrane associated with F-actin) and (b) actin cables
(bundles of F-actin; Adams and Pringle, 1984
; Mulholland
et al., 1994
). In mitotically dividing cells, cortical actin
patches cluster in the growing bud, and actin cables
aligned along the mother-bud axis are well positioned to
deliver mitochondria to the daughter cell (Kilmartin and
Adams, 1984
). Mitochondria have been shown to colocalize with actin cables in yeast, and some mutations in actin
result in abnormal mitochondrial morphology, distribution, and motility (Drubin et al., 1993
; Lazzarino et al.,
1994
; Simon et al., 1995
). In addition, recent studies established that isolated yeast mitochondria bind reversibly to phalloidin-stabilized actin filaments in vitro (Lazzarino et
al., 1994
). These mitochondria were shown in a related assay to contain a myosin-like actin-dependent motor activity on their surface (Simon et al., 1995
). Based on these results, it has been suggested that yeast mitochondria are
transported from the mother cell into the emerging bud
using actin filaments as "tracks" and a myosin-like motor
activity on the surface of the organelle.
Materials and Methods
. Yeast mating, sporulation, tetrad dissection, complementation studies, and meiotic segregation analysis were performed
using standard genetic techniques (Sherman et al., 1986
). The lithium acetate method was used for all yeast transformations (Ito et al., 1983
) and
gene disruption experiments (Rothstein, 1991
; Baudin et al., 1993
).
Escherichia coli strains DH5
and JM109 (Promega, Madison, WI) were
used for bacterial manipulations of clones and plasmids. Molecular cloning techniques were performed as described by Maniatis et al. (1982)
.
Identification of mdm Mutants
The wild-type strain FY10 (Winston et al., 1995) was UV mutagenized
(25% survival), and a collection of 4,000 temperature-sensitive yeast strains
was generated. To identify mitochondrial distribution and morphology
(mdm) mutants in this collection, individual strains were grown for 16 h at
the permissive temperature (25°C) in 500 µl of YPD, diluted 1:10 into 500 µl
fresh YPD, and shifted to the nonpermissive temperature (37°C) for 3 h.
100 µl of the culture was stained with a final concentration of 100 nM 3,3
dihexyloxacarbocyanine (DiOC6) (Molecular Probes, Eugene, OR), and
mitochondria were visualized by fluorescence microscopy. 18 mdm mutant
strains were identified that produced large buds lacking DiOC6-stained mitochondria. Standard genetic methods were used to show that the mdm
phenotype in each strain was due to a single recessive mutation. In all but
one case, the mdm phenotype was linked to the temperature-sensitive growth defect in three or more backcrosses to the wild-type parent. The
exception was mdm29, which exhibited only a mitochondrial morphology
defect. Complementation analysis was performed between the 18 mdm
mutants identified in this screen and the existing mdm and mmm mutants
generously provided by M. Yaffe (University of California, San Diego)
(McConnell et al., 1990
; Sogo and Yaffe, 1994
) and R. Jensen (Johns Hopkins University, Baltimore, MD) (Burgess et al., 1994
). One mutation was
allelic to the previously identified mdm2/ole1 gene (Stukey et al., 1989
,
1990
; Stewart and Yaffe, 1991
). The remaining 17 mdm mutants define 10 new complementation groups designated mdm20-mdm29.
Cloning, Sequencing, and Disruption of MDM20 and Identification of TPM1 as an Unlinked Suppressor
An mdm20-1 strain (GHY1) that had been backcrossed three times to the
wild-type parent strains FY10 and FY22 was transformed with a yeast genomic library contained within the low copy plasmids YCp50 (Rose et al.,
1987) (obtained from the American Type Culture Collection, Rockville,
MD) and p366 (kindly provided by T. Formosa, University of Utah, Salt
Lake City). 12,000 Ura+ transformants containing the YCp50 library were
tested for complementation of the temperature-sensitive growth defect in
the mdm20-1 strain. 14 colonies contained rescuing plasmids. Restriction
digest and sequence analysis showed that these strains contained six different overlapping genomic inserts. The plasmid A6-2p, containing a 9-kb genomic insert, was selected for further analysis. A 1.6-kb BsaBI/KpnI fragment from A6-2p inserted into pRS416 (low copy CEN plasmid) or
pRS426 (multicopy 2µ plasmid) (Stratagene, La Jolla, CA) digested with
KpnI and SmaI was sufficient for complementation of the temperaturesensitive growth defect in mdm20-1 cells. The sequence of a large genomic region containing this fragment was released as part of the Yeast Genome
Sequencing Project (GenBank accession number X86470), and the 1.6-kb
fragment was shown to contain only the TPM1 gene. Integrative mapping
(Rose and Broach, 1991
) revealed that mdm20 is not linked to TPM1.
Thus, TPM1 is an unlinked extra copy suppressor of the mdm20 mutation.
The MDM20 gene was isolated by transforming the mdm20-1 strain
GHY1 with the p366 genomic library. Of the 23,000 Leu+ transformants
screened, 24 contained plasmids that could rescue the temperature-sensitive growth defect in mdm20-1 cells. Of these 24 plasmids, restriction digestion and Southern analysis revealed that seven contained TPM1. The
remaining 17 plasmids contained four different genomic inserts that
shared common overlapping restriction fragments. Plasmid A15-5p contained a 5.2-kb SphI fragment that, when cloned into YCp50, was sufficient to fully complement the mdm20-1 mutation. The DNA carried by
this plasmid was sequenced on both strands using an ABI373 automated
sequencer at the University of Utah Health Sciences Sequencing Facility (supported by National Cancer Institute grant 5-P30CA42014). Deletion mapping and transposon mutagenesis (Sedgwick and Morgan, 1994) revealed that a 2,388-bp open reading frame was responsible for complementation. A Pfu polymerase (Stratagene) generated a PCR fragment
containing the open reading frame, and 500 bp of 5
and 3
flanking sequence was subcloned into the EagI and SalI sites of pRS416 and pRS426.
The two resulting plasmids complemented both the temperature-sensitive
growth defects and mitochondrial inheritance defects in mdm20-1 cells.
The wild-type sequence of the MDM20 gene inserted into both plasmids
was verified by sequence analysis. Meiotic segregation analysis showed
that the cloned open reading frame (MDM20) mapped to the mdm20-1
mutation. The predicted Mdm20 protein sequence was compared with all
available databases using the FASTA (Pearson and Lipman, 1988
), BLAST
(Altschul et al., 1990
), and Prosite (Bairoch et al., 1995
) programs. No significant homologies were detected. The putative coiled-coil domains in
the Mdm20p were found using the COILS 2.1 program (Lupas et al.,
1991
). The MDM20 GenBank accession number is U54799.
To generate the mdm20 null mutation (mdm20), a 1.9-kb LEU2 PCR
fragment was subcloned into pRS406-MDM20 digested with HindIII and
SpeI, replacing 2,219 bp (codon 12-751) of the MDM20 open reading
frame with LEU2. Digesting this plasmid with SalI and EagI released a
2.9-kb fragment containing the LEU2 gene bordered by MDM20-flanking
sequences that was used to transform the diploid yeast strain JSY948. The
mdm20
::LEU2 disruption was confirmed by Southern blotting of genomic DNA isolated from a Leu+ transformant. Tetrad analysis of sporulated diploids confirmed that the LEU2 marker cosegregated 2:2 with
mdm20 phenotypes (temperature sensitivity and defective mitochondrial
inheritance) and that cells harboring the mdm20
mutation were viable at
25°C. To document the mitochondrial inheritance defect in the mdm20
strain, wild-type (JSY999) and isogenic mdm20
(JSY1065) cells were
stained with DiOC6 and examined microscopically as described below.
Suppression of the Temperature-sensitive and Organelle
Inheritance Defects in mdm20 Cells
To examine the suppression of the mdm20 temperature-sensitive growth
defect by TPM1, the wild-type (JSY999) or isogenic mdm20
(JSY1065)
strains harboring pRS426, pRS426-MDM20, or pRS426-TPM1 were grown
to log phase at 25°C in SD minus uracil (SD
Ura) liquid medium. Equal
numbers of cells were then serially diluted and spotted on SD
Ura solid
media and grown at 37°C for 3 d. To examine the suppression of the
mdm20
temperature-sensitive growth defect by TPM2, the wild-type
(JSY999) or isogenic mdm20
(JSY1065) strains harboring pRS416,
pRS416-MDM20, or GAL1-TPM2 (pEH006; a generous gift from E. Harsay and A. Bretscher, Cornell University, Ithaca, NY) were grown to log
phase at 25°C in SGal
Ura liquid medium. Equal numbers of cells were
then serially diluted and spotted on SGal
Ura solid media and grown at
37°C for 3 d.
To determine the effects of extra copies of TPM1 and TPM2 on the mitochondrial and nuclear inheritance defects in mdm20 cells, the wildtype (JSY999) or mdm20
(JSY1065) strains harboring pRS416 or pRS426,
pRS426-TPM1, or GAL1-TPM2 were grown in SGal
Ura or SD
Ura
liquid media for 16 h at 25°C, diluted, and grown in log phase at 25° or
37°C for 3 h. Mitochondrial inheritance was evaluated by DiOC6 staining
as described above. Nuclear segregation was analyzed by 4
,6-diamidino2-phenylindole staining (DAPI) as described previously (Pringle et al., 1991
).
In each experiment, at least 400 cells were counted. tpm1
(JSY707) cells
were examined for defects in mitochondrial and nuclear inheritance using
the same protocol.
Characterization of Mdm20p-HA Expression
To monitor Mdm20p levels, the protein was tagged by the addition of
three hemagglutinin (HA) epitopes at the amino and carboxy termini.
A 3.1-kb SalI/HpaI fragment from pRS416-MDM20 was inserted into
p-ALTER-1 (Promega) digested with SalI and SmaI to create p-ALTER1-MDM20. Site-directed mutagenesis (Altered Sites II; Promega) was
used to insert NotI sites immediately downstream from the initiating Met
or the carboxy-terminal Lys of MDM20. An NotI fragment from plasmid
GTEP1 containing three tandem HA epitopes was inserted into the
NotI sites at the 5 or 3
ends of MDM20. The correct orientation was
verified by sequence analysis. MDM20-N-HA and MDM20-C-HA SalI/
KpnI fragments were inserted into pRS416 and pRS426 digested with SalI
and KpnI to create pRS416-MDM20-N-HA, pRS426-MDM20-N-HA,
pRS416-MDM20-C-HA, and pRS426-MDM20-C-HA. All of the MDM20HA constructs fully rescued the temperature-sensitive growth defect, the
mitochondrial inheritance defect, and the loss of actin cables in mdm20
cells (JSY1065), indicating that the fusion proteins are functional.
To detect the Mdm20p-HA fusion proteins, 108 cells from log phase
cultures were harvested and lysed using 0.2-mm glass beads in 500 µl of
SDS-PAGE sample buffer. 25 µl of each lysate was loaded onto an 8%
SDS-PAGE gel, and, after electrophoresis, the proteins were transferred
to nitrocellulose. Western blot analysis was performed using standard protocols (Harlow and Lane, 1988). Mdm20p-HA fusion proteins were detected with polyclonal rabbit antibodies against HA (1:1,000) (BAbCO,
Richmond, CA). Detection was carried out using the ECL kit (New England Nuclear, Boston, MA). The fusion proteins encoded by the
MDM20-N-HA and MDM20-C-HA constructs have a predicted molecular mass of 97 kD but migrated with an apparent molecular mass of 90 kD
on SDS-PAGE gels. Since the amino- and carboxy-terminal HA-tagged
Mdm20p gave identical results, the aberrant size is likely not due to proteolysis, but instead may result from some structural feature or posttranslational modification of the fusion proteins. Comparison of Mdm20p-HA
levels was performed using NIH Image 1.60 (National Institutes of Health, Bethesda, MD).
Synthetic Interactions Involving mdm20
The effects of combining mdm20 with tpm1
or tpm2
mutations were
determined by constructing diploids heterozygous for mdm20
and
tpm1
(JSY1138) or mdm20
and tpm2
(JSY1374). The tpm1
mutation was generated by transforming the wild-type strain FY22 with a PCR fragment containing 50 bp of TPM1 flanking sequence interrupted by the
HIS3 gene using the technique described by Baudin et al. (1993)
. The disruption removes all but 42 bp of the 3
TPM1 coding region. The disruption in JSY707 was verified by Southern analysis. The tpm2
disruption
was constructed in JSY999 using the TPM2 disruption plasmid pBD103 (a
gift from A. Bretscher) as described previously (Drees et al., 1995
) to produce the tpm2
::HIS3 strain JSY1285. The tpm2
::HIS3 disruption was
verified by Southern analysis. The heterozygous diploids JSY1138 and
JSY1374 were sporulated, and tetrads were dissected. The tpm1
::HIS3
mdm20
::LEU2 mutants germinated and gave rise to microcolonies containing 50-100 cells. In separate experiments, tpm1
::HIS3 mdm20
::
LEU2 double mutants were recovered when JSY1138 diploids containing
the wild-type MDM20 gene on a URA3 plasmid were sporulated and dissected. The synthetic growth defect of mdm20
tpm1
double mutants was
verified by showing that these cells were unable to lose the plasmid when grown on 5-FOA-containing medium. The JSY1374 diploid gave rise to
viable mdm20
::LEU2 tpm2
::HIS3 double mutants with no obvious synthetic growth defects. Crosses to test possible synthetic interactions between mdm20
::LEU2 and bem2-10 (Wang and Bretscher, 1995
), myo2-66 (Johnston et al., 1991
), and sac6
::LEU2 (Adams et al., 1991
) were performed essentially as described above.
Analysis of the Actin Cytoskeleton in mdm20 and
tpm1
Cells
To visualize F-actin, the wild-type (JSY999) or mdm20 (JSY1065) strains
containing pRS426 were grown 16 h at 25°C in SD
Ura liquid medium.
The cultures were then diluted (to 2 × 106 cells per ml) into fresh SD
Ura and grown at 25° or 37°C for 3 h. F-actin was detected with rhodamine-phalloidin (Molecular Probes) as described previously (Adams
and Pringle, 1991
). To determine the effects of overexpressing TPM1 and
TPM2 on the actin cytoskeleton in mdm20
mutants, the mdm20
strain
JSY1065 carrying pRS426-TPM1 or GAL1-TPM2 was grown in SD
Ura or SGal
Ura at 25° or 37°C as described above, and then stained
with rhodamine-phalloidin. To analyze the effects of Mdm20p-HA overexpression on actin organization in tpm1
cells, the tpm1
strain JSY707
carrying pRS426, pRS426-MDM20, or pRS426-MDM20-C-HA was grown
and stained as described above.
Microscopy
Cells were viewed on an Axioplan microscope using a ×100 Plan-neofluor
(NA 1.3) objective (Carl Zeiss, Inc., Thornwood, NY) using an optivar
setting of ×1.6, a 200-W mercury lamp, and the following excitation wavelengths: DiOC6 (450-490 nm), DAPI (365 nm), and rhodamine (546 nm).
Differential interference contrast (DIC) and fluorescence digital images
were captured and assembled into figures as described previously (Roeder
and Shaw, 1996). Images were printed on a Tektronix Phaser IIsdx dyesublimation printer (Wilsonville, OR).
mdm20 Mutants Exhibit Defects in Mitochondrial Inheritance
To identify yeast genes required for mitochondrial inheritance, we generated and screened a collection of temperature-sensitive mutants for strains that failed to transport
mitochondria into growing buds. Individual strains grown
at 25°C were shifted to 37°C for 3 h and stained with the lipophilic, fluorescent dye, DiOC6, under conditions that
preferentially label yeast mitochondria (Pringle et al.,
1989; Shaw and Wickner, 1991
; Koning et al., 1993
). 18 of
the 4,000 mutants examined exhibited defects in mitochondrial distribution and/or morphology. The mutations
in these strains were recessive in heterozygous diploids
and segregated 2:2 in backcrosses with the wild-type parent strain. 17 of these strains fell into ten complementation
groups designated mdm20-mdm29; the remaining mutation was a new allele of the previously characterized gene
MDM2/OLE1 (Stukey et al., 1989
, 1990
; Stewart and Yaffe, 1991
). In all but one mutant (mdm29), the temperaturesensitive growth defects were linked to the defects in mitochondrial distribution and morphology. The MDM20 complementation group, defined by seven mutant alleles, was
chosen for further study.
Wild-type strains grown at 25° or 37°C (Fig. 2, A and B)
segregate a portion of the mitochondrial network into
buds almost as soon as they can be detected on the surface
of the mother cell. In contrast, mdm20 mutants retained
their branched mitochondrial networks but produced
large buds that lack this organelle (Fig. 2, C and D). This
mitochondrial inheritance defect was observed at the permissive temperature and became more pronounced at 37°C (Table II). Both transmission EM and DAPI staining of
mitochondrial genomes confirmed that mitochondria were
absent from mdm20 buds (data not shown). In addition,
organelles labeled with a mitochondrially targeted form of
the green fluorescent protein (kindly provided by R. Jensen) also failed to be transported into buds in the mdm20 strain (data not shown). Although the mdm20 mutation
caused a striking mitochondrial inheritance defect, it did
not severely affect metabolic functions of mitochondria
since they could still be efficiently labeled with the potential-dependent dye DiOC6, which only stains actively respiring organelles (Pringle et al., 1989).
Table II. Mitochondrial Inheritance in mdm20 and tpm1 Mutants |
Isolation and Sequence Analysis of the MDM20 Gene
The MDM20 gene was isolated by complementing the
temperature-sensitive growth defect of the mdm20-1 mutant allele (see Materials and Methods). Integrative mapping studies indicated that the cloned DNA contained the
wild-type MDM20 gene. Transposon mutagenesis (Sedgwick and Morgan, 1994) and DNA sequence analysis revealed that a 3.2-kb fragment (Fig. 3 A) was sufficient to
rescue both the temperature-sensitive growth defect (Fig.
4) and the mitochondrial inheritance defect (not shown) in
the mdm20 mutant strain.
The MDM20 gene predicts a novel, hydrophilic protein
that contains 796 amino acids with a calculated molecular
mass of 92,821 daltons (Fig. 3 B). The sequences adjacent
to the first potential initiating methionine (Fig. 3 B, asterisk) fit the consensus for a translational initiation site in
yeast (Cigan and Donahue, 1987). Moreover, we demonstrated that an in-frame epitope tag (HA) inserted immediately downstream of this methionine is translated and
can be detected on a Western blot (data not shown). Comparison of the Mdm20 protein sequence with all available
databases using the FASTA (Pearson and Lipman, 1988
),
BLAST (Altschul et al., 1990
), and Prosite (Bairoch et al.,
1995
) algorithms revealed no significant homologies with
other proteins. However, two potential heptad repeat-
containing regions located in the carboxy-terminal portion
of the polypeptide are predicted to adopt an
-helical coiled-coil structure (Fig. 3 B, boldface amino acids). Heptad repeats have been implicated in the homo- and heterodimerization of a variety of proteins with diverse functions (Cohen and Parry, 1986
, 1990
).
Mdm20p Is Required for Mitochondrial Inheritance during Budding but Does Not Alter Mitochondrial Morphology
Yeast cells harboring mdm20-1 through mdm20-7 mutations exhibited defects in mitochondrial inheritance, grew slowly compared to wild type at 25°C, and were dead at 37°C. To further evaluate the role of MDM20 in vivo, we generated a null allele by replacing codons 12-751 with the LEU2 gene (Fig. 3 A). When diploids heterozygous for the mdm20::LEU2 null allele were sporulated, dissected into tetrads, and incubated at 25°C, all four spores in each tetrad germinated. However, spores lacking MDM20 grew slowly and formed small colonies relative to wild type. Further analysis indicated that spores containing the mdm20:: LEU2 disruption did not grow on fermentable (dextrose) or nonfermentable (glycerol) carbon sources at 37°C.
The mitochondrial inheritance defect in the mdm20::
LEU2 cells (mdm20) was similar to that observed for the
original seven mdm20 mutant alleles. In log phase cultures
grown at 25°C, 14% of mdm20
mother cells remained attached to buds that failed to inherit mitochondria (Table
II). In contrast, mitochondrial segregation defects were
not observed in wild-type cultures grown at 25°C (Table
II). Incubation at 37°C for 3 h resulted in an increased fraction of mdm20
cells exhibiting mitochondrial inheritance defects (58%), whereas mitochondrial partitioning in
wild-type cells did not change significantly (<1%) (Table
II). Moreover, when mdm20
cells arrested in the unbudded stage were released upon temperature shift, >90% of
the buds that formed at 37°C did not inherit mitochondria
(data not shown). Despite the severe defect in mitochondrial transmission to buds, DiOC6-stained mitochondrial networks appeared wild type in the mdm20
cells at both
25°C (98% wild type) and 37°C (95% wild type) (see Fig.
2 D). Thus, MDM20 is required for normal mitochondrial
inheritance in yeast but does not appear to play an essential role in maintaining the reticulated network of mitochondrial membranes.
Although nuclear inheritance was normal in mdm20
cells grown at 25°C, a small number (5%) of binucleate
cells was observed at 37°C (Table III; discussed below).
This defect in nuclear segregation, while significant, is
much less severe than the defect in mitochondrial inheritance in the mdm20 mutant. We also examined the distribution of the vacuole in the mdm20 mutant. We found
that, at both 25° and 37°C, new mdm20
buds contained
vacuolar material even when mitochondria were absent
from the buds (data not shown). Thus, mutations in the
mdm20 gene appear to have the most dramatic affect on
inheritance of the mitochondrial compartment.
Table III. Nuclear Segregation in mdm20 and tpm1 Mutants |
Extra Copies of Genes Encoding the Actin Binding Proteins Tpm1p and Tpm2p Partially Rescue Mitochondrial Inheritance Defects and Temperature-sensitive Growth Defects in the mdm20 Mutant
To identify loci that interact genetically with MDM20 and
to learn more about the role of the Mdm20 protein, we analyzed multicopy suppressors of the mdm20-1 temperature-sensitive growth defect. The multicopy suppressors
were isolated from a genomic library in a centromerebased yeast vector at the same time the MDM20 gene was
cloned (see Materials and Methods). One of the clones we
isolated contained TPM1, a previously identified gene that
encodes the actin binding protein tropomyosin (Liu and
Bretscher, 1989). Tropomyosins are rod-shaped coiled-coil
dimers that bind along the groove of the actin helix. Skeletal tropomyosin modulates the interaction between actin
and myosin during muscle contraction. In yeast, however,
tropomyosins are thought to function in the assembly and/
or stabilization of actin cables (Liu and Bretscher, 1989
; Bretscher et al., 1994
). Although TPM1 is not an essential
gene, cells lacking TPM1 grow slowly, are heterogeneous
in size, and are often multinucleate due to defects in aligning the mitotic spindle (Liu and Bretscher, 1992
; Palmer
et al., 1992
; Wang and Bretscher, 1995
). Loss of TPM1 also
results in severe defects in actin cytoskeletal organization,
most notably the loss of actin cables (see below) (Liu and
Bretscher, 1989
). In addition to TPM1, yeast contain a second tropomyosin encoded by the TPM2 gene (Drees et al.,
1995
). Disruption of the TPM2 gene does not visibly affect the organization of the actin cytoskeleton and does not
hamper cell growth (Drees et al., 1995
). However, the genetic and biochemical behavior of Tpm2p and the observed synthetic lethality between tpm1 and tpm2 mutations indicate that cellular functions of these two proteins
overlap (Drees et al., 1995
).
Extra copies of the TPM1 gene provided on a low copy
number (not shown) or high copy number plasmid partially rescued the temperature-sensitive lethality in mdm20
cells grown at 37°C (Fig. 4). In contrast, the conditional lethality of the mdm20
mutation was completely suppressed by a wild-type copy of the MDM20 gene (Fig. 4).
Extra copies of TPM1 also suppressed mitochondrial inheritance defects in the mdm20
strain. In a culture of
mdm20
cells harboring TPM1 on a multicopy plasmid,
the fraction of cells lacking mitochondria in buds was reduced from 14% to 2% at 25°C and from 58% to 17% at
37°C (Table II). These results indicated that the Tpm1
protein could functionally substitute for the loss of the
Mdm20 protein.
To determine whether functional overlaps also existed
between Mdm20p and Tpm2p, we asked whether extra
copies of TPM2 could rescue mutant phenotypes in mdm20
cells. As shown in Fig. 4, the temperature-sensitive growth
defect of mdm20
cells was partially suppressed when
Tpm2p was overexpressed from the GAL1 promoter (Fig.
4 B). Overexpression of Tpm2 was also sufficient to reduce the mitochondrial inheritance defect in mdm20
from 14% to 9% at 25°C and from 58% to 34% at 37°C
(Table II). Thus, Mdm20p and Tpm2p apparently have
some overlapping functions as well.
MDM20 Is Essential for the Integrity of Actin Cables in Yeast
Taken together, the data presented above suggested that
(a) MDM20 and TPM1 participate in overlapping, essential cellular functions; and (b) Tpm2p can partially substitute for Mdm20p when overexpressed. Given what is known
about the function of tropomyosins (Pittenger et al., 1994),
these results also suggested that the integrity of the actin
cytoskeleton is important for mitochondrial inheritance
during yeast budding, and that the mdm20 mutation affects the assembly or organization of F-actin. To further
investigate this possibility, we examined the actin cytoskeleton in mdm20 null cells by rhodamine-phalloidin staining.
At both 25° and 37°C, wild-type cells contained well-
defined actin cables and cortical actin patches concentrated in growing buds (Fig. 5, A-D). In contrast, actin cables
were absent in 100% of the mdm20 null cells examined at
both temperatures (Fig. 5, E-H). mdm20
cells were able
to divide, however, and contained brightly staining cortical
patches that were predominantly clustered in buds at 25°C
(Fig. 5, E and F; >95% of cells) and partially delocalized
at 37°C (Fig. 5, G and H; >50% of cells). The fact that mitochondrial inheritance defects are already present at 25°C
in the mdm20 mutant (at a temperature where patches are
still properly localized) suggests that it is the disruption of
actin cables that is primarily responsible for the lack of mitochondrial transmission.
Rhodamine-phalloidin staining also revealed that multiple copies of TPM1 restored actin cable formation in the
mdm20 mutant. At 25°C, >95% of the mdm20 cells containing TPM1 on a multicopy plasmid had actin cables that
were robust and extended the full length of the mother cell
(Fig. 5, I and J). However, these restored cables appeared
fewer in number than those observed in wild type. At
37°C, >95% of mdm20 cells also contained the TPM1-
restored cables. However, these cables were shorter than
normal, and, while visible near the mother-bud neck, they
rarely extended the full length of the mother cell (Fig. 5, K
and L). The delocalization of actin cortical patches in
mdm20 cells at 37°C was also rescued by introducing extra copies of TPM1 (Fig. 5, K and L; >95% of cells). Abbreviated actin cables were also observed in >90% of the
mdm20
cells overexpressing Tpm2p from the GAL1 promoter at 25°C (Fig. 5, M and N). At 37°C, only faint cables
were observed near the mother-bud neck in mdm20
cells
containing GAL1-TPM2 (Fig. 5, O and P; >90% of cells).
Finally, the wild-type MDM20 gene on a low copy number
plasmid was able to completely restore cables in >98% of
mdm20
cells (data not shown). This partial restoration of
actin cables and mitochondrial inheritance by TPM1 and
TPM2 was striking and suggested that the defect in mitochondrial inheritance observed in mdm20 is linked to the
loss of actin cables in these cells.
MDM20 Fails to Complement Mutant Phenotypes
in tpm1 Cells
Although overexpression of TPM1 suppressed mitochondrial inheritance defects and restored actin cables in the
mdm20 mutant, the functions of the Tpm1 and Mdm20
proteins were not completely interchangeable. As shown
in Fig. 6, C and D, and reported previously, actin cables
are absent in tpm1 mutant cells (Liu and Bretscher, 1989
).
However, actin cables could not be restored by introducing extra copies of the MDM20 gene into tpm1
cells on a
high copy number plasmid (Fig. 6, E and F) or by overexpressing epitope-tagged versions of the Mdm20p (Fig. 6, G
and H; data not shown). In the latter experiments, Mdm20p
overexpression was monitored using amino- and carboxyterminal HA-tagged Mdm20 proteins (see Materials and
Methods). Wild-type cells containing Mdm20p-C-HA on a
centromere-based plasmid expressed relatively low levels
of the tagged protein (Fig. 7, lane 3). The steady state protein level increased more than eightfold when Mdm20-CHA protein was expressed from a multicopy plasmid (Fig.
7, lane 4). Identical results were obtained when expression
of the Mdm20p-N-HA was examined in wild-type cells (data
not shown). Fusion of the HA tag to the Mdm20 protein
had no obvious effects on its function, as these constructs
completely rescued temperature-sensitive growth defects,
mitochondrial inheritance defects, and loss of actin cables
in mdm20 mutant strains (data not shown). Furthermore,
overexpression of HA-tagged Mdm20p constructs did not
induce additional phenotypes in wild-type cells (data not
shown). We found that tpm1
cells overexpressing Mdm20p
(Fig. 7, lane 8) did not grow significantly better than tpm1
cells alone. In addition, overexpression of Mdm20p did
not rescue the lethality observed in tpm1
tpm2
double
mutants. Together, these findings suggest that MDM20
cannot bypass the requirement for Tpm1p and Tpm2p in
cells. Furthermore, although expression of Tpm1p in wildtype cells results in thicker actin cables (Liu and Bretscher,
1989
), the actin cytoskeleton was not affected by overexpressing Mdm20p in a wild-type strain (data not shown).
Thus, Mdm20p and Tpm1p appear to perform some distinct functions in cells.
Loss of Actin Cables in mdm20 and tpm1
Cells Disrupts Mitochondrial Inheritance and
Nuclear Segregation to Different Extents
To further evaluate functional overlaps between Mdm20p
and Tpm1p, we examined mitochondrial inheritance and
morphology in the tpm1 mutant. Although actin cables
are also absent in tpm1
cells, we were surprised to find
that tpm1 null strains did not exhibit significant defects in
mitochondrial inheritance at 25° (<1%) or 37°C (5%) (Table II). In addition, mitochondrial morphology appeared
normal in tpm1
cells at both temperatures (99% wild type at 25°C and 96% wild type at 37°C). The mitochondrial inheritance phenotype of tpm1
contrasted with that
of mdm20 null cells, which displayed more severe defects
in mitochondrial inheritance at both temperatures (14% at
25°C and 58% at 37°C; Table II). These phenotypic differences, together with the results described above, supported
the notion that the Mdm20 and Tpm1 proteins perform some distinct roles in cells. To extend these observations,
we examined nuclear segregation (a process known to be
defective in tpm1 mutants) in isogenic tpm1 and mdm20
strains.
During division, the mitotic spindle is oriented by interactions of astral microtubules with the actin cytoskeleton.
Disruption of this interaction in act1 mutants results in misoriented spindles that give rise to binucleate cells (Palmer
et al., 1992). Consistent with previous reports (Liu and
Bretscher, 1989
; Wang and Bretscher, 1995
), we found
that tpm1
mutants lacking actin cables exhibited nuclear
segregation defects and produced a significant proportion of multinucleate cells at 25°C (13%) and 37°C (16%) (Table III). Conversely, nuclear segregation was wild type in
mdm20
cells grown at 25°C, although a small number
(5%) of binucleate cells was observed at 37°C (Table III).
Extra copies of TPM1 (but not overexpression of Tpm2p)
suppressed the formation of binucleate cells at 37°C in the
mdm20
strain (Table III). Thus, tpm1 mutants displayed
more severe defects in nuclear segregation than mdm20 mutants. Together, these data indicate that, although TPM1
and MDM20 are both required for the formation and/or
stabilization of actin cables, their roles in cellular processes such as mitochondrial inheritance and nuclear segregation differ significantly.
Null Mutations in mdm20 are Synthetically Lethal With Mutations in tpm1, myo2, and bem2
Although TPM1 and TPM2 null mutants are alive at 25°C,
the combinatorial loss of these two genes in a haploid
strain results in cell death (Drees et al., 1995). This synthetic lethality is thought to arise because Tpm1p and
Tpm2p carry out some redundant functions required for
an essential cellular process (Drees et al., 1995
). The similar actin phenotypes we observed in tpm1 and mdm20 mutants prompted us to genetically test the possibility that
MDM20 acts in a common pathway with tropomyosins.
The phenotypes of haploid mdm20
tpm1
and mdm20
tpm2
double mutants were examined after dissecting tetrads generated from diploid cells heterozygous for null
mutations in both MDM20 and TPM1. In 33 tetrads analyzed, double mdm20
tpm1
mutants were never observed (30 expected; Table IV). Although mdm20
tpm1
spores germinated, they were defective in mitotic growth
and gave rise to microcolonies of 50-100 cells that could
not be analyzed further. These results were confirmed by
repeating the cross with an mdm20
strain carrying the
wild-type MDM20 gene on a URA3-marked plasmid. In
this experiment, mdm20
tpm1
cells harboring the
MDM20 URA3 plasmid were recovered and were viable
unless forced to lose the plasmid on 5-FOA plates (data
not shown). Synthetic lethal interactions were not observed between MDM20 and TPM2 in similar crosses (Table IV), and mitochondrial inheritance and morphology
defects were not observed in tpm2
cells (data not shown).
Table IV. Synthetic Lethal Relationship Involving mdm20 |
Previous studies indicated that tpm1 also exhibits synthetic growth defects with mutations in BEM2 (Wang and
Bretscher, 1995) and MYO2 (Liu and Bretscher, 1992
).
The BEM2 gene encodes a GTPase-activating protein required for bud emergence, a process that involves polarization of actin cables and patches to the site of bud growth
(Kim et al., 1994
; Peterson et al., 1994
). MYO2 encodes a
type V myosin family member that forms a cap at or near
the plasma membrane on unbudded cells and small buds
(Johnston et al., 1991
; Lillie and Brown, 1994
). In crosses
similar to those described above, we determined that mutations in BEM2 and MYO2 are also synthetically lethal
with mdm20 (Table IV). We also examined synthetic interactions between mutations in MDM20 and the SAC6
gene that encodes the actin cross-linking protein, fimbrin
(Adams et al., 1991
). Although Sac6p, like Tpm1p, localizes to actin cables in wild-type yeast cells, synthetic
growth defects were not detected for tpm1 sac6 double
mutants (Adams et al., 1993
) and were not observed in
crosses we performed with mdm20 and sac6 mutant strains
(Table IV). Thus, mdm20 and tpm1 mutants not only exhibit similar actin organization defects but also show the
same pattern of genetic interactions.
We have demonstrated that the MDM20 gene encodes a novel protein required for proper mitochondrial segregation in yeast. Cells lacking Mdm20p are temperature sensitive for growth and fail to transport mitochondria into newly formed buds. Our results indicate that the defect in the mdm20 mutant specifically disrupts mitochondrial transport but not mitochondrial morphology in these cells. In addition, the mdm20 mutation does not severely interrupt the division and segregation of the nucleus, and other cytoplasmic organelles, such as vacuoles, are always detected in mdm20 daughter cells that fail to inherit the mitochondrial compartment. Together, our findings establish an essential role for MDM20 in mitochondrial partitioning during mitotic division.
Two different cytoskeletal elements in yeast, actin (Drubin et al., 1993; Lazzarino et al., 1994
) and an intermediate
filament-like protein (McConnell and Yaffe, 1992
), have
been proposed to play a central role in mitochondrial
inheritance. In this study we present two lines of in vivo
evidence that mitochondrial inheritance in yeast is an actin-mediated process. First, two major phenotypic consequences of disrupting MDM20 appear to be the cessation
of mitochondrial movement into buds during division and
the loss of observable actin cables in cells. Second, overexpression of two well-characterized actin binding proteins,
Tpm1p and Tpm2p, suppresses temperature-sensitive growth
and mitochondrial inheritance defects and partially restores actin cables in the mdm20 mutant. Although it is
possible that Mdm20p fulfills distinct functions in mitochondrial inheritance and actin cable organization, the observation that overexpression of Tpm1p and Tpm2p can
partially rescue defects in both processes in mdm20 mutants suggests that these two phenotypes cannot be separated from one another. Moreover, a direct link between
mitochondrial segregation and the actin cytoskeleton is
consistent with the recent observations that yeast mitochondria colocalize with actin cables in vivo (Drubin et al., 1993
), can bind to phalloidin-stabilized actin filaments in
vitro (Lazzarino et al., 1994
), and contain an actin-dependent myosin-like motor activity on their surface (Simon et al.,
1995
). Thus, our data strongly support a model in which
mitochondria are transported into yeast buds along polarized actin filaments or cables.
The organization and stabilization of the actin cytoskeleton in yeast depends on the activities of a large number of
actin binding proteins and regulatory factors. Mdm20p is a
new member of this important group of proteins required
for the integrity of actin cables in cells. Previous studies
indicate that defects in actin organization cause a variety
of phenotypes including temperature-sensitive lethality,
osmotic sensitivity, and defects in cell morphology, mitochondrial dynamics, secretion, endocytosis, and nuclear
segregation (for review see Bretscher et al., 1994; Welch
et al., 1994
). In addition to the phenotypes we have reported here for the mdm20 mutant, our preliminary studies suggest that mdm20 cells are rounder than wild type
and heterogeneous in size, exhibit defects in chitin localization, and accumulate small vesicles (unpublished observations). These data provide further support that MDM20
is required for normal functions of the actin cytoskeleton. Most importantly, MDM20 defines a new class of genes
that control both actin organization and mitochondrial
transport during division.
Previous studies of the actin-myosin complex identified
a myosin "footprint" on the actin monomer (Rayment et al.,
1993; Schroder et al., 1993
). Charge-to-alanine substitutions located under the equivalent myosin footprint in the
yeast actin monomer have been shown to cause defects in
mitochondrial morphology, specifically mitochondrial aggregation (Drubin et al., 1993
). The mutants with aberrant
mitochondrial morphology exhibit severe actin organization defects that are most pronounced at 37°C, including
loss of actin cables and/or patches, delocalized patches,
and reduced or faint cables. In contrast, we find that
mdm20 mutants lacking actin cables exhibit disrupted mitochondrial transport but not mitochondrial morphology.
Similarly, we do not observe defects in mitochondrial morphology in isogenic tpm1 mutant cells. If the actin cytoskeleton plays a role in regulating mitochondrial morphology, then the structures required must still be present in
mdm20 and tpm1 mutant cells. Alternatively, other cytoplasmic structures or cytoskeletal proteins may be responsible for controlling yeast mitochondrial morphology.
Our observation that mitochondrial morphology and inheritance is normal in the tpm1 mutant is interesting in
light of previous reports that tpm1
strains generate petites (lose mitochondrial genome function) at a higher frequency than wild type (Liu and Bretscher, 1992
). We also
find that mdm20
and tpm1
cells generate petites at a
high frequency when maintained on dextrose. One possible explanation for these results is that tpm1 daughter cells
frequently receive DNA-free mitochondrial compartments.
In our experiments, mitochondrial morphology and distribution were measured by labeling the mitochondrial compartment with the potential dependent dye, DiOC6, and
labeling mtDNA nucleoids with DAPI. We observed that tpm1
cells segregated both the mitochondrial compartment (Table II) and mitochondrial nucleoids (data not
shown) into daughter cells. Furthermore, we did not detect a large number of tpm1 cells lacking mt nucleoids.
Thus, the increased petite formation in tpm1 cells is not
simply the result of a block in mtDNA transfer to buds.
Further experiments are required to determine the mechanism by which these strains become petite.
Some of our studies suggest that Tpm1p and Mdm20p
might perform overlapping functions required for the integrity of the actin cytoskeleton. The disruption of both
genes causes a similar loss of actin cables in cells and combinations of mutations in MDM20 and TPM1 result in synthetic lethality. In addition, like tpm1, mdm20 exhibits synthetic growth defects in combination with mutations in
either BEM2 or MYO2 but not SAC6 (Fig. 8). Furthermore, we observe that overexpression of Tpm1p restores
actin cables and rescues mitochondrial inheritance defects
in mdm20. However, this suppression is not reciprocal;
overexpression of Mdm20p does not rescue mutant phenotypes in tpm1 cells, suggesting that their roles in organizing actin differ. Mdm20p and Tpm1p do not appear to
be structurally homologous since their amino acid sequences and sizes are quite different. If Mdm20p and
Tpm1p do not have redundant functions, then an alternative explanation for the rescue of mdm20 mutant phenotypes by overexpressed Tpm1p is required. One possibility
is that the overexpression of Tpm1p leads to the global
stabilization of all actin filaments and cables in mdm20 cells, including those necessary for mitochondrial transport and inheritance. In support of this model, overexpression of Tpm1p is reported to cause more prominent cables
and actin networks in wild-type cells and can restore actin
cables in act1-2 mutant strains (Liu and Bretscher, 1989).
Although overexpression of Tpm2p also suppresses mutant phenotypes in mdm20, we did not observe synthetic
lethality in mdm20 tpm2 double mutants. Previous studies showed that the level of Tpm2p expression in wild-type
cells is much lower than that of Tpm1p, and that cells lacking TPM2 do not exhibit defects in actin organization or
growth (Drees et al., 1995
). Thus, mdm20
tpm2
cells
may contain enough Tpm1p to compensate for the loss of
Tpm2p and prevent the cell death observed in mdm20
tpm1
double mutants.
Interestingly, although mutations in MDM20 and TPM1
cause similar defects in actin organization, the mutant phenotypes in these two strains are distinct. mdm20 mutant
cells exhibit severe defects in mitochondrial inheritance
(58%) and only slight defects in nuclear segregation (5%).
Conversely, tpm1
strains exhibit weak defects in mitochondrial inheritance (5%) and stronger defects in nuclear
segregation (16%). As discussed above, while overexpression of Tpm1p can rescue mutant phenotypes in mdm20,
the converse is not true. These observations suggest that
Mdm20p and Tpm1p perform different roles in vivo and
support the hypothesis that there are functionally distinct
classes of actin-containing structures in cells. It is important to note that mdm20 and tpm1 mutant cells lacking actin cables may contain individual actin filaments that are
not detected by rhodamine-phalloidin staining. Thus, actin filaments that play a role in mitochondrial inheritance may
be present in the tpm1 mutant but absent in the mdm20
mutant. By the same reasoning, actin-containing structures required for nuclear segregation may be more severely disrupted in the tpm1 mutant than in the mdm20
mutant. In this way, MDM20 and TPM1 could be acting to
establish molecular and functional heterogeneity in the actin cytoskeleton.
As illustrated in Fig. 8, our synthetic lethal studies suggest that MDM20 functions in a cellular process that also
requires TPM1, BEM2, and MYO2. Assembly and/or stabilization of the actin cytoskeleton is an obvious candidate
for this process since defects in actin organization have
been reported for mutations in all of these genes (Liu and
Bretscher, 1989; Johnston et al., 1991
; Kim et al., 1994
;
Wang and Bretscher, 1995
). The synthetic growth defects
we observe between mdm20 and tpm1, bem2, and myo2
may simply reflect the fact that partial defects in actin organization can be tolerated at 25°C, but combinations of
defects cannot. However, this interpretation is not supported by the findings that double mutants lacking both
MDM20 and SAC6 (Table IV and Fig. 8) or SAC6 and
TPM1 (Adams et al., 1993
) are viable. An alternative possibility is that synthetic lethality between mutations in these genes results from a failure to coordinate bud site assembly with the actin polarization required for directed membrane transport and bud growth. Lillie and Brown (1994)
have suggested that Myo2p localized at the incipient bud
site might function to anchor actin filaments that are required for the polarized delivery of vesicles to the bud. In
support of this model, both myo2 and tpm1 mutants accumulate small vesicles, and we have observed similar vesicles in a small number of mdm20 cells (data not shown).
Our studies of the mdm20 mutant indicate that polarized
actin cables are also required for the delivery of mitochondria to buds. Physical and genetic interactions reported for
BEM2 suggest that the Bem2p protein may also localize to
the bud site where it is postulated to regulate Tpm1p-containing actin filaments (Wang and Bretscher, 1995
). Based
on the synthetic lethal interactions observed to date, we
speculate that viable mdm20 and tpm1 cells lacking actin cables still contain some undetected actin filaments that
are properly polarized to the bud site. However, when
mdm20 and tpm1 are combined with mutations in genes
that control actin filament polarization to the bud site, synthetic lethality results.
Although MDM20 encodes a novel protein required for
the organization of the actin cytoskeleton, analysis of the
predicted Mdm20 amino acid sequence does not reveal
any known actin binding domains. Mdm20p does contain
two potential heptad repeats, however, which could modulate its homo- or heterodimerization through the formation of -helical coiled-coils. While the specific biochemical activity of Mdm20p is unknown, it is likely to participate in the assembly or function of actin-containing structures
necessary for mitochondrial segregation. In this regard,
Mdm20p could bind directly to filamentous actin or might
act in a signaling pathway that directs the assembly or stabilization of actin filaments or cables that transport mitochondria during cell division. We think it is unlikely that
Mdm20p is a major structural component of actin filaments or cables for two reasons. First, our studies with the
HA-tagged Mdm20p suggest that relatively low levels of the protein are able to completely rescue mutant phenotypes in the mdm20 strain (see Fig. 7). Second, we have
been unable to localize the low abundance of HA-tagged
Mdm20p in wild-type or mdm20 cells (data not shown). In
cells overexpressing HA-tagged Mdm20p, the protein is
found dispersed throughout the cytoplasm and does not
appear to be concentrated along actin cables or at actin
patches (data not shown). Based on these results, we suggest that Mdm20p serves a regulatory function in cells. We
are currently studying the function of this interesting protein in organizing actin and in directing mitochondrial
transport and inheritance.
Received for publication 23 October 1996 and in revised form 6 February 1997.
Please address all correspondence to Janet M. Shaw, Department of Biology, University of Utah, Salt Lake City, UT 84112. Tel.: (801) 585-6205. Fax: (801) 581-4668.We are grateful to Drs. Alison Adams, Anthony Bretscher, Susan Brown, John Cooper, Tim Formosa, Edina Harsay, Rob Jensen, Sue Lillie, David Stillman, Fred Winston, and Michael Yaffe for providing strains, antibodies, and plasmids. We especially thank Jason Singer and William Bleazard for the mdm20/sac6 and mdm20/bem2 synthetic lethality data. We also thank David Nix for technical advice, and Drs. Mary Beckerle, Tim Formosa, David Gard, and members of the Shaw laboratory for stimulating discussions and careful review of the manuscript.
This work was supported by grants from the American Cancer Society (CB-97) and the National Institutes of Health (NIH) (GM53466) to J. Shaw. G. Hermann was supported in part by an NIH Predoctoral Genetics training grant and a University of Utah Graduate Research fellowship.
DAPI, 4,6-diamidino-2-phenylindole;
DIC, differential interference contrast;
DiOC6, 3,3
dihexyloxacarbocyanine;
5-FOA, 5-fluoro-orotic acid;
HA, hemagglutinin;
SD, synthetic dextrose;
SGal, synthetic galactose;
Ura, uracil.