Previous Article | Next Article 
Molecular and Cellular Biology, September 2001, p. 6044-6055, Vol. 21, No. 17
Institute of Medical Microbiology,
Immunology, and Hygiene, Technical University of Munich, D-81675
Munich, Germany
Received 28 November 2000/Returned for modification 20 March
2001/Accepted 23 May 2001
The mechanism of cargo coupling to kinesin motor proteins is a
fundamental issue in organelle transport along microtubules. Kinectin
has been postulated to function as a membrane anchor protein that
attaches various organelles to the prototype motor protein kinesin. To
verify the biological relevance of kinectin in vivo, the murine
kinectin gene was disrupted by homologous recombination. Unexpectedly,
kinectin-deficient mice were viable and fertile, and no gross
abnormalities were observed up to 1 year of age. The assembly of the
endoplasmic reticulum was essentially unaffected in kinectin-deficient
cells. Mitochondria appeared to be correctly distributed throughout the
cytoplasm along the microtubules. Furthermore, the stationary
distribution and the bidirectional movement of lysosomes did not depend
on kinectin. Kinectin-deficient phagocytes internalized and cleared
bacteria, indicating that phagosome trafficking and maturation are
functional without kinectin. Thus, these data unequivocally indicate
that kinectin is not essential for trafficking of lysosomes,
phagosomes, and mitochondria in vivo.
Microtubule (MT)-dependent membrane
transport is essential for a variety of cellular processes (for a
review, see references 22 and 46). MT-dependent
intracellular transport processes are mediated by motor proteins of the
kinesin and of the cytoplasmic dynein superfamilies. These
molecules act as mechanochemical adenosin triphosphatases, converting
chemically bound energy into directed motile force along the MT tracks.
The majority of the kinesin family members are anterograde motors,
conveying their cargoes specifically toward the plus ends of the MT.
Some kinesin family members and cytoplasmic dynein function as
retrograde motors, mediating cargo transport toward the MT minus ends
(reviewed in references 21 and 54). Since the first
description of kinesin (6, 56), approximately 30 members
of murine kinesin superfamily proteins (KIFs) have been identified
(21, 34, 59). Genetic inactivation of various KIFs and of
the cytoplasmic dynein heavy chain (cDHC) in the mouse and in
Drosophila melanogaster resulted in embryonic or perinatal
lethality, thus proving the vital importance of these motor proteins
(14, 18, 38, 44, 51, 52, 60). A conventional kinesin
consists of two kinesin heavy chains (KHCs) and two kinesin light
chains (KLCs). The KHC binds directly to the MT via its globular
N-terminal head (23, 45). The C-terminal regions of the
KHC associate with the KLCs and are thought to interact with the
cargoes (50). Recently, the KLCs have been implicated in
the regulation of motor activity. Up to now, it has not been clarified,
whether KLCs are directly involved in cargo binding (9, 12,
49).
While many KIFs have been identified and much has been learned about
kinesin functions (reviewed by Goldstein and Philip [16] Hirokawa et al. [22]), there is only scarce information
available concerning the receptors anchoring the various KIFs to their
cognate cargoes. Kinectin (KNT), the first proposed candidate anchor
protein for kinesin tails on vesicle membranes, was purified by
affinity column chromatography (53). The KHC binding
domain of KNT was mapped to a short C-terminal KNT region.
Correspondingly, the KNT interaction domain in kinesin was defined to
reside in the KHC tail (39). KNT associates with membranes
via its N terminus (13, 61). It is an integral membrane
protein of ca. 160 kDa, located at the cytoplasmic face of membranous
vesicles (53, 61). KNT can form heterodimers with a
shorter 120-kDa isoform, presumably by interaction of To analyze the biological relevance of KNT in cells and in animals, the
murine knt gene was disrupted by homologous recombination in
embryonic stem (ES) cells. KNT knockout mice were viable, reproduced normally, and did not develop any obvious abnormalities for up to 1 year of age. KNT-null mutant cells showed a normal assembly of
endoplasmic reticulum (ER) and cis-Golgi, and the stationary intracellular distribution of mitochondria and lysosomes was
unaffected. The lack of KNT did not abrogate lysosome motility.
Peritoneal exudate cells (PEC) obtained from knt-deficient
mice were capable of phagocytosing and eliminating Escherichia
coli bacteria, indicating that phagosome trafficking and
maturation occur in the absence of KNT.
Targeting vector and structure of the genomic knt
locus.
A partial human cDNA (the kind gift of M. Krönke) was
used to screen a mouse 129Sv/J genomic library in
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.17.6044-6055.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Intact Lysosome Transport and Phagosome Function
Despite Kinectin Deficiency
and
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
-helical
coiled coils that encompass the C-terminal two-thirds of the molecule
(27). However, the function of the 120-kDa isoform is
unclear. Antibody inhibition studies suggested a participation of KNT
in MT-dependent vesicle motility. An anti-KNT antibody raised against a
native epitope in the KNT cytoplasmic domain was shown to efficiently
block plus-end-and; to a lesser extent, also minus-end-directed vesicle
motility in an in vitro trafficking assay (28). The same
antibody was also reported to reduce kinesin binding to motile vesicles
(28). Furthermore, attempts to suppress KNT function by
peptide inhibition approaches suggested a requirement for KNT in
phagosome and lysosome motility. Here, peptides derived from the
central KNT stalk domain but not from the KNT C terminus were described
to block bidirectional movement of phagosomes in vitro
(3). In this study, the reported content of KNT was
elevated on late phagosomes of higher motility. In a different study,
overexpression of the KNT-kinesin binding domain was shown to disrupt
anterograde lysosome transport (39). However, it remains
controversial whether KNT is an essential anchor for kinesin on cargo
membranes (21).
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
DASH II. A 14.5-kb genomic clone hybridizing to the 5' region of the cDNA was isolated, mapped, and sequenced. It contained exons 2 to 6 and in part exon 7, corresponding to nucleotide (nt) 
12 to nt 1163 of the published murine cDNA (GenBank accession no. L43326). The sequenced exons were
identical to the murine knt coding sequence. The ATG start site was located at nt 19 in exon 2. The exon borders were as follows:
exon 2 (nt 12 to 548), exon 3 (nt 549 to 686), exon 4 (nt 687 to
860), exon 5 (nt 861 to 991), exon 6 (nt 992 to 1108), and exon 7 (nt
1109 to >1163). To insert loxP signals into intron 2 and
intron 5 of the knt locus, a targeting vector was
constructed as follows (Fig.
1A). A synthetic
loxP motif and a PstI and a BglII site
were added by PCR to a 0.7-kb genomic DNA fragment located directly 3'
to a unique MfeI site of the genomic clone. This 0.7-kb
fragment was inserted into a modified pBluescript vector (Stratagene)
using PstI and BamHI to generate the plasmid kntSA. A 1.7-kb fragment containing exon 2 was excised from the genomic
clone with NcoI and KpnI and inserted into pGEM7
(Promega) cut with SmaI and KpnI. The 1.7-kb
fragment was recovered from this plasmid by digestion with
EcoRI and ClaI and ligated to kntSA cut with
EcoRI and ClaI to create kntSAL1. The genomic
region containing exon 3 to exon 5 was inserted into kntSAL1 cut with KpnI and EcoRI as a 9.2-kb
KpnI/MfeI fragment, yielding kntLS. The targeting
vector kntTV was completed by inserting a
PGK-neor gene flanked by loxP motifs
into the KpnI site and the HSV-tk cassette
into the SalI site of kntLS, respectively. The
orientations of loxP motifs were verified by
restriction analysis and sequencing.
View larger version (80K):
[in a new window]
FIG. 1.
Construction of the KNT targeting vector and generation
of mutant mice. (A) Schematic representation of the genomic
knt locus, the targeting construct (kntTV) and the different
mutated alleles. Homologous recombination of kntTV introduces a
loxP-flanked neomycin resistance gene (neo) into
intron 2 and a single loxP motif into intron 5 of the
knt genomic locus. Cre-mediated recombination at
the targeted locus (T) produces either a floxed knt allele
(F) or a deleted knt allele ( 
) by excision of the
neomycin resistance gene or by deletion of the neomycin
resistance gene together with exons 3 to 5, respectively. Exons are
depicted as shaded boxes; loxP motifs are indicated as
filled triangles. Transcriptional directions of neomycin
resistance and tk (open boxes) are indicated by arrows. fl3,
3' external probe; neo1, neo probe; E, EcoRV; P,
PstI; C, ClaI; S, SacI; N,
NcoI; K, KpnI; M, MfeI; M/EI,
MfeI/EcoRI. (B) Southern blot analysis of genomic
DNA from targeted ES cell clones before and after in vitro
Cre recombination (left) and from mouse tail biopsies
(right). A 1.8-kb restriction fragment after PstI digestion
is diagnostic for the mutated alleles in contrast to a 2.6-kb fragment
generated from the wild-type allele. Note that the deleted allele is
cut at an endogenous PstI site and not at the
PstI site introduced with the distal loxP motif.
EcoRV digestion generates fragments of 8.5 kb (), 11.2 kb
(T), and 17.7 kb (wt and F) in size. Southern detection of the
PstI and the EcoRV digests was performed with the
external probe fl3. Hybridization with neo1 after
ClaI/SacI double digestion yields one 12-kb
fragment for the targeted allele (T), indicating a single integration
event. E14, genomic DNA from E14.1 ES cells.
Targeting of the knt locus and generation of KNT
mutant mice.
For conditional targeting approaches, cointegration
of a third, distal loxP motif, together with a floxed marker
gene, into the target locus is crucial. Since there is no selection
pressure on integration of the distal loxP motif,
cointegration can be very inefficient, especially if the distance to
the floxed marker cassette is long (1). To enable direct
screening for correct recombination of the single loxP site,
the targeting vector kntTV was linearized near the single
loxP motif with NotI and transfected into
embryonic day 14.1 (E14.1) ES cells. ES cell transfection, culture and
selection was done as described previously (41). 288 G418-
and ganciclovir-resistant ES cell colonies were picked and screened for
integration of the single loxP motif by PCR using the
external primer knt-S1 (5'-GAACAGATCCACATCACATCC-3') and the internal primer knt-LF (5'-CCAATTCCTGCAGAGATCTATAAC-3'),
which binds to genomic, polylinker, and loxP sequences
and is therefore specific for the single loxP motif. Of 29 PCR positive clones, 11 were analyzed by Southern blotting of genomic
DNA. The correct recombination event could be verified for 10 of 11 clones by blotting ES cell DNA after digestion with EcoRV or
PstI and hybridization with the 3' flanking probe fl3.
Specifically, the PstI digest was indicative for
cointegration of the single loxP site, whereas the
EcoRV digest was used to analyze the correct localization of
the floxed neomycin resistance gene. Single-copy integration was verified by Southern probing a ClaI/SacI
double digest of the ES cell DNA with a part of the neomycin
resistance cassette. ES cell clones carrying a floxed (F)
knt allele were generated by deleting the neomycin
resistance gene from the original targeted (T) knt
locus in vitro. After transient transfection of 20 µg of supercoiled
pIC-Cre plasmid (17), G418-sensitive ES cell clones were selected and characterized by PCR and Southern analysis for
the different deletion events. The frequencies of
Cre-mediated deletion yielding the floxed and the deleted
alleles were 6 and 2%, respectively. Chimeric mice were generated from
knt+/T and knt+/F ES
cells by injection of C57BL/6 blastocysts and CD1 morula aggregation. Chimeric mice obtained from knt+/T ES cell lines
were crossed to the Cre-transgenic deleter strain (47), resulting in deletion of the neomycin resistance
gene and exons 3 to 5 of the knt gene
(knt+/
). Germ line transmission of the
targeted and the floxed allele, as well as successful deletion, were
identified by Southern blot analysis. Mice were housed in an animal
facility with barrier conditions.
Construction of pkntegfpN20. A full-length murine knt cDNA was isolated from a brain endothelioma cell library by screening with a human knt cDNA and then ligated into an EcoRI/SmaI-cut pEGFP-N1 vector (Clontech) to create pkntegfpN20. The knt cDNA contained the alternatively spliced "inserted sequences" 1 and 4, but not sequences 2, 3, and 5, as confirmed by sequencing (30).
RNA and protein analysis.
Total RNA was extracted as
described elsewhere (42). For Northern blotting, 20 µg of RNA was separated on a formaldehyde agarose gel,
transferred onto Genescreen Plus nylon membrane (DuPont), and
hybridized with the following 32P-labeled murine cDNA
probes: knt3', knt5' (encompassing the murine cDNA from nt 1250 to 4180 and from nt 43 to 1950, respectively) and glctrp (1.6-kb fragment of
the murine facilitated glucose transporter, GenBank accession no.
M22998) as a loading control. Reverse transcription-PCR (RT-PCR)
analysis was performed with the primers knt#p12
(5'-GAGTCAACTGCTTACAGCGC-3'), knt#p13
(5'-CCCCTTATTCATGCAACTAC-3'), knt#p68
(5'-CCTTGAAGAGCAGGTCATC-3'), knt#p69
(5'-AAGGAGAACTGAGTGGTC-3'), and knt#p70
(5'-GATCTTTCATTCTTGCTA-3') located in exons 6, 4, 2, 6, and
7, respectively. With the indicated combinations of primers, wild-type
and deleted alleles give rise to products of the following sizes:
knt#p68 + knt#p12 
716 and 273 bp, knt#69 + knt#70 165 and 165 bp, and knt#p13 + knt#p12 400 bp and no
product (due to deletion of exon 4).
) allele.
Phagocytosis assays.
PEC were obtained by peritoneal lavage
from mice challenged with thioglycolate (Sigma) for 4 days. Then,
5 × 105 PEC were incubated with 2.5 × 107 yellow-green fluorescent FluoSpheres (2 µm; Molecular
Probes F-8827) for 5 to 240 min at 37°C. As a negative control cells were left on ice for 60 min. PEC were separated from
unincorporated beads by density centrifugation through fetal calf
serum (FCS) (360 relative centrifugal force [RCF], 10 min),
washed, and fixed in 1% paraformaldehyde. Cytospins were assayed by
confocal microscopy. For analysis of phagosome function, PEC were
challenged with bacteria. Overnight cultures of Escherichia
coli DH5 transformed with GFPmut2 (expressing a GFP mutant
suitable for fluorescence-activated cell sorting detection
[8], The kind gift of H. Häcker) and of untransformed controls were washed three times with phosphate-buffered saline (PBS) and adjusted to an optical density at 600 nm of 1. A
volume of 2.5 ml of the bacterial suspensions was added to
106 PEC in 10 ml of Dulbecco modified Eagle medium,
supplemented with 10% fetal calf serum, and 0.1% 2-mercaptoethanol
(all from Gibco), and 100 U of penicillin per ml, 100 U of streptomycin per ml, and 2 nM L-glutamine. After 1 h of incubation,
the PEC were washed and centrifuged at 240 REF three times to remove
free bacteria. After a further 1, 4, and 17 h, PEC were washed
with PBS, fixed in 2% formalin, and analyzed by flow cytometry.
Lysosome assay. Lysosome motility was analyzed according to the method of Heuser (20). In brief, embryonic fibroblasts (EF) were removed from the CO2 incubator, washed three times for 15 min with Ringer's solution (R; 155 mM NaCl, 5 mM KCl, 2 mM CaCl2, 1 mM MgCl2, 2 mM NaH2PO4, 10 mM HEPES buffer [pH 7.2], 10 mM Glucose, 0.5 mg of bovine serum albumin [BSA] per ml), stained for 5 min with 330 nM Mitotracker in R, washed briefly, and incubated without CO2 at 37°C for 30 min. Cells were then transferred to NH4Cl R (BR; 30 mM NH4Cl in R), acetate R (AR; 80 mM NaCl, 70 mM sodium acetate, 5 mM KCl, 2 mM CaCl2, 1 mM MgCl2, 2 mM NaH2PO4, 10 mM HEPES buffer [pH 6.9], 10 mM glucose), or R alone for 60 min. Subsequently, cells were fixed with 2% paraformaldehyde-0.1% glutaraldehyde in PBS for 10 min at ambient temperature and then processed for immunofluorescence. For the rebound experiments, cells were incubated in BR for 30 min, washed three times in R, and incubated for 30 min in AR before fixation. For quantification, lysosome localization was scored for one of three possibilities: clustered, distributed, or peripheral. One hundred cells per sample were analyzed microscopically without knowing the treatment and genotype of the cell samples.
Immunocytochemistry.
EF were obtained from embryos of the
different genotypes as described previously (42). EF were
grown overnight on glass slides, fixed with 2% paraformaldehyde-0.1%
glutaraldehyde in PBS for 10 min at 37°C, permeabilized with 1%
saponin in PBS for 10 min at 37°C, and blocked with 5% skim
milk powder in PBS for 30 min at room temperature, followed by 1-h
incubations at room temperature with primary and secondary antibodies
diluted with 1% skim milk in PBS. Each incubation step was followed by
brief washing steps. Mouse anti- tubulin (1:200, clone DM 1A;
Sigma), mouse anti-gm130 (1:400, clone 35: Transduction Laboratories), rabbit anti-KNT (1:100; RS-TUM), or rat anti-LAMP-1 fluorescein isothiocyanate (FITC; 1:200, clone 1D4B; PharMingen)
were used as primary antibodies and detected with Alexa488- or
Alexa546-labeled goat anti-mouse IgG; immunoglobulin G
(1:200; Molecular Probes) or HRP-conjugated goat anti-rabbit IgG
(1:1,000; Bio-Rad) secondary antibodies. HRP development was performed
as described earlier (42). Cells were observed through a
Leica DMRBE microscope or a Zeiss 410 confocal microscope. For labeling
of the ER, cells were fixed with ice-cold ethanol (95%)-acetic
acid (5%) for 1.5 min, blocked for 30 min with 8% BSA in PBS,
and incubated with rabbit anticalreticulin (1:100; Upstate) and
Alexa546-conjugated goat anti-rabbit IgG (1:200; Molecular Probes)
antibody in 1% BSA-PBS.
| |
RESULTS |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Generation of knt/ and
kntF/F mice.
The targeted disruption of
various KIFs resulted in embryonic or perinatal lethality (38,
51, 52, 60). KNT was postulated to be a major kinesin-binding
protein contained in motile vesicles (53). Thus, a
targeted knt-null mutation could be assumed to be fatal.
Therefore, a conditional targeting strategy (17) based on
the Cre/loxP recombination system was employed to inactivate the knt gene. The targeting vector was constructed in a way
that a loxP flanked neomycin resistance gene and a third,
distal, loxP site were inserted into intron 2 and intron 5 of a genomic knt fragment, respectively (Fig. 1A). The
herpes simplex virus thymidine kinase (tk) gene was included
to enable negative selection against random integrants. Linearization
of the targeting construct close to the neomycin resistance cassette
used for positive selection may result in a high proportion of clones
with correct recombination of the floxed neomycin resistance marker
but without cointegration of the distal loxP motif (1,
29). (T. Plitz and K. Pfeffer, unpublished data). Therefore, the
targeting vector was linearized at the 3' end near the distal
loxP motif and transfected into E14.1 ES cells
(41). Transfectants were selected with G418 and ganciclovir, and double-resistant clones were screened for correct integration of the distal loxP motif by PCR (see Materials
and Methods). Correct homologous recombination encompassing all three loxP motifs could be confirmed by genomic Southern blot
analysis in 10 of 11 ES cell clones tested (Fig. 1B. data not shown).
To obtain ES cell clones carrying a floxed (F) knt allele,
the floxed neomycin resistance gene was removed from the targeted (T)
locus by transient Cre transfection. Chimeric mice were
generated from ES cell clones harboring the targeted or the floxed
knt allele. Chimeras harboring the targeted knt
allele were bred with transgenic "deleter" mice expressing
Cre recombinase in early development (47). This
cross gave rise to mice heterozygous for the deleted knt
() allele. Germ line transmission of the targeted (T), the floxed
(F), and the deleted () alleles was proven by Southern blot analysis
(Fig. 1B).
), as well as
knt+/F control mice, were intercrossed to
produce homozygous offspring. Both crosses gave rise to litters of
normal size, with wild-type, heterozygous
(knt+/ or knt+/F), and
homozygous (knt/ or
kntF/F) offspring present at a frequency
consistent with Mendelian inheritance (data not given).
knt/ and kntF/F
animals appeared healthy and reproduced normally. Gross pathological examination of mice up to 1 year of age did not reveal abnormalities.
The deleted knt allele is a null allele.
To verify
that the targeting resulted in a knt null mutation, KNT
expression was analyzed in knt/ mice.
Cre-mediated deletion between the outer loxP
sites results in excision of a genomic region encompassing exons 3 to 5 of the knt gene. The deletion leads to direct splicing from
exon 2 to exon 6, thus generating a frameshift mutation that results in a premature termination codon (PTC). Therefore, putatively, a truncated protein consisting of the N-terminal 178 amino acids of KNT
might be translated. However, such a putative truncated KNT protein
would lack the interaction domain with kinesin (39). Using
RT-PCR, the engineered splicing of exon 2 directly to exon 6 in the
knt transcripts could be identified in
knt/ EF, but not in wild-type EF controls
(Fig. 2A). Sequencing of these RT-PCR
products was employed to verify the expected exon 2 to exon 6 join in
the knt/ transcripts (Fig. 2A). In
general, a mutation generating a PTC in an upstream exon leads to rapid
degradation of the mRNA by a mechanism known as nonsense-mediated
decay (reviewed by Hentze and Kulozik [19]).
Consistently, by using knt cDNA probes that cover the entire
coding sequence, knt mRNA could not be detected in
knt/ EF by Northern blot analysis. Both
cDNA probes, however, hybridized to the knt transcripts
contained in wild-type RNA (Fig. 2B). As predicted from these results,
no KNT protein was detected in knt/ mice,
as verified by Western blot analysis of tissue homogenates from
different organs (Fig. 2C) or immunolabeling of KNT in EF (Fig. 2D).
However, KNT was readily detectable in protein extracts from
kntF/F mice, indicating that the insertion of
loxP sites into introns of the knt locus did not
affect KNT biosynthesis. These data prove that KNT was successfully
inactivated in knt/ mice.
|
Subcellular localization of KNT.
To establish the subcellular
compartmentalization of KNT, fibroblasts were transiently transfected
with pkntegfpN20, encoding a murine N-terminal KNT-eGFP fusion protein.
The resulting expression of green fluorescent protein (GFP)-tagged KNT
enables the detection of cellular compartments associated with KNT.
Confocal microscopy of pkntegfpN20-expressing cells revealed a
reticular, perinuclear staining pattern (Fig.
3A), corresponding to previous reports using anti-KNT antibodies (13, 53). This result
establishes a correct localization of the exogenously expressed eGFP
fusion protein. Calreticulin and gm130 can be used as ER and
cis-Golgi markers, respectively (40)
(35). In the transfected cells, KNT-eGFP almost
exclusively colocalized with the ER and not with the Golgi compartment
(Fig. 3B and D). Virtually no colocalization of KNT-eGFP was detectable
with microtubules (Fig. 3E) identified by labeling with
anti--tubulin antibody (4). KNT-eGFP was restricted to
the perinuclear region in almost all inspected cells. Pronounced
KNT-eGFP staining in the cell periphery, implying the association of
KNT with anteriogradely transported organelles, could not be detected.
Only in very few heavily overexpressing cells, KNT-eGFP was found as a
punctate staining pattern in the periphery (Fig. 3F and G). This label
may also colocalize with ER structures, since the ER is known to extend
to the cell periphery (31). These data confirm that KNT is
almost exclusively targeted to the ER.
|
KNT deficiency does not alter the stationary localization of
membrane organelles.
Since KNT was postulated to be a
kinesin-binding protein that is required for kinesin-based vesicle
motility (28), knt/ EF were
analyzed for a possible transport defect of membrane organelles.
Labeling of the ER with an anti-calreticulin antibody resulted in a
perinuclear reticular staining pattern in
knt/ and knt+/+
cells (Fig. 4J and E). The ER structures
seemed equally large and spread out in cells of both genotypes,
indicating that the assembly of the ER is independent from KNT. This is
intriguing since KNT predominantly localizes to the ER (Fig. 3B). In
the null mutant EF the perinuclear, tubular staining pattern of the cis-Golgi apparatus with an anti-gm130 antibody was
indistinguishable from the gm130 staining pattern in wild-type cells
(Fig. 4I and D).
|
/ cells were radially arranged and
stretched out along microtubules (Fig. 4A to C and F to H). These data
indicate that KNT is not required for the transport of mitochondria
along and attachment of these organelles to the cytoskeleton.
KNT is dispensable for anterograde lysosome transport in EF.
Like mitochondria, lysosomes are attached to and move along
microtubules (20). Lysosome localization can be
synchronized by pharmacological treatments, thus facilitating the
analysis of lysosome transport in vivo (20). Cytoplasmic
alkalinization induced by NH4Cl treatment of the cells
causes lysosomes to cluster around the nucleus, while cytoplasmic
acidification achieved by acetate treatment leads to dispersion of the
lysosomes throughout the cytoplasm, eventually resulting in their
accumulation at the very edge of the cell. The dependence of
anterograde lysosome transport on kinesin has been shown in cells
expressing a rigor neuronal kinesin mutant or in cells lacking KIF5B
(36, 52). Furthermore, a recent report suggested an
involvement of KNT in lysosome trafficking (39). To test
lysosome motility in the absence of KNT, lysosomes were localized by
labeling with anti-LAMP-1 antibody (7) in
knt/, kntF/F, and
knt+/+ EF after incubation in ringer (R)
solution or in basic R (BR) or acidic R (AR). Staining of mitochondria,
which do not redistribute during pH changes (20), was
included to monitor the integrity of cells during treatment. In 95.5%
of the control EF incubated in R, lysosomes were dispersed throughout
the cytoplasm (Fig. 5A and B and Table
1). This stationary distribution of lysosomes was nearly
identical in knt/ EF. Here, a dispersed
lysosome localization was observed in 92% of the cells (Fig. 5C and D
and Table 1). Perinuclear clustering of lysosomes upon alkalinization
in BR occurred similarly in control and null mutant cells, resulting in
clustered lysosomes in more than 85% of both cell types (Fig. 5E to H
and Table 1). Acidification in AR induced centrifugal motility of
lysosomes in knt/ and
knt+/+ EF, causing peripheral accumulation of
lysosomes in 77 and 88.5% of the cells, respectively (Fig. 5lF to
L and Table 1). During these experiments,
kntF/F EF were undistinguishable from wild-type
control or knt/ cells (Table 1). To
further analyze anterograde lysosome transport, cells were treated
with BR and subsequently transferred to AR. Redistribution of
initially clustered lysosomes to the cell periphery could be observed
in knt/ EF, as well as wild-type control
EF (Fig. 6). The fraction of cells with
redistributed lysosomes was identical with 97.7% for the null mutant
and 97% for the wild-type cells (Table
2). These data prove that kinesin-driven
anterograde transport of lysosomes in EF does not depend on KNT.
|
|
|
|
PEC show full phagocytic capacity despite the absence of KNT.
Cells can internalize large particulate matter by phagocytosis. After
their formation at the plasma membrane, phagosomes are delivered to the
prelysosomal compartment, where they mature to phagolysosomes
(43). The extensive trafficking necessary to enable the
interaction of phagosomes with lysosomes in the perinuclear area to
form the phagolysosome is microtubule dependent (11, 25).
The bidirectional movement of phagosomes along microtubules was shown
to be mediated by cytoplasmic dynein and kinesin and could be inhibited
by KNT peptides (3). Furthermore, KNT was reported
localizing on phagosomes and, compared to early phagosomes, elevated
KNT protein levels were described on late phagosomes of higher motility
(3). To test the contribution of KNT to the maturation and
function of phagosomes, PEC obtained from
knt/ and control mice were analyzed for
their phagocytic capacity. In a first set of experiments, PEC were
incubated with fluorescent latex microspheres. Both,
knt/ and knt+/
PEC phagocytosed the beads without differrences in kinetics or efficiency (Fig. 7A and data not shown).
Especially after longer incubation periods, PEC of both genotypes were
loaded with many beads, accumulating inside the cell (Fig. 7A, insets).
To provide a more physiological substrate for phagocytosis and to
enable the examination of phagosome maturation and function, PEC were challenged with E. coli expressing GFP. The uptake and the
elimination of the GFP-labeled bacteria by PEC were monitored by flow
cytometry. It could be detected that the bacteria were rapidly taken
up, and more than 80% of the PEC were GFP+ after 10 min.
After 60 min, more than 98% of the PEC of both genotypes had
incorporated bacteria (data not shown). During a following 24-h chase
period, the fluorescence of the PEC decreased as they degraded the
GFP+ bacteria (Fig. 7B). In this assay system,
knt/ PEC were undistinguishable from
knt+/+ controls with respect to the kinetics and
efficiency of phagocytosis and the clearance of E. coli
bacteria. These data imply that cellular trafficking enabling the
formation of fully functional phagolysosomes is not impaired in the
absence of KNT.
|
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
Kinesin-driven intracellular membrane transport is of vital
importance for a large variety of cellular processes, yet how cargoes
are coupled to the kinesin motors is still ill defined. KNT
has been proposed to attach cargoes to the prototypic motor protein conventional kinesin (16). The present
study describes a novel mouse mutant deficient in KNT.
Unexpectedly, KNT-deficient mice appear healthy and fertile.
Detailed analysis of knt/ mice reveals
that KNT cannot be considered to function as a general anchor
for the kinesin-driven transport of mitochondria, lysosomes, or phagosomes.
At present, there are conflicting reports about the involvement of kinesin in Golgi-to-ER transport. Redistribution of Golgi markers to the ER could be induced by brefeldin A treatment in conventional KHC (kif5B)-null mutant cells (52). In contrast, injection of anti-kinesin antibody into cells or inhibition of KHC expression by antisense oligonucleotide suppression blocked this Golgi-ER redistribution (31, 52). Additionally, there is evidence that establishment and placement of the ER inside the cell are driven by kinesins (10, 55), although these processes might not be dependent on KIF5B (52). Disruption of the knt gene (this study) apparently does not affect ER and cis-Golgi morphology. These data provide evidence that ER assembly does not depend on KNT or, alternatively, that the kinesin motors needed for ER integrity do not bind to KNT.
Two murine KIFs, KIF1B and KIF5B, have been implicated in the movement
of mitochondria (37) (52). Both KIFs
associate with mitochondria. While evidence for an involvement of KIF1B mainly came from in vitro trafficking assays, genetic inactivation experiments clearly demonstrated that transport of mitochondria in
intact cells requires KIF5B. In KIF5B-null mutant cells obtained from
extraembryonic membranes, mitochondria clustered perinuclearly. Ectopic
reconstitution of KIF5B expression in kif5B
/
cells resulted in a dispersion of mitochondria. In contrast, in
knt/ EF cells, mitochondria were not found
around the nucleus but were distributed throughout the cytoplasm and
aligned along MT, thus indicating that KNT does not contribute to
mitochondrion motility. Provided that there is no synergistic use of
motors other than KIF5B to drive anterograde mitochondrion transport in
EF, it could be suggested that KNT does not anchor conventional KHC.,
i.e., KIF5B, to mitochondria.
The bidirectional transport of phagosomes has been reported to depend
on KNT (3). Additionally, the increased motility of late
phagosomes has been attributed to the accumulation of KNT on phagosomes
over time, suggesting a contribution of KNT to phagosome maturation
(3). However, knt/ PEC are
fully able to phagocytose and clear E. coli bacteria, providing evidence for the conclusion that the trafficking and maturation of phagosomes can occur in the absence of KNT. In the study
by Blocker et al. (3), peptide inhibition was chosen to
suppress KNT function. Fragments of KNT were produced in bacteria, purified, and added to an in vitro system reconstituting phagosome transport. In this assay, two fragments derived from the central part
of the KNT protein (encompassing residues 295 to 612 and 568 to 943)
blocked the bidirectional movement of phagosomes, whereas a third,
C-terminal KNT fragment (residues 924 to 1321) had no effect. One of
the central KNT fragments (residues 568 to 943) is recognized by a
monoclonal anti-KNT antibody that interferes with the motility of
microsome preparations in vitro (3, 28). The conclusion
that the central KNT coiled-coil region is indispensable for phagosome
transport is contradictory in the light of a recent study
characterizing the interacting domains of KNT and kinesin (39). Here, the kinesin-binding domain was mapped to a
short region (residues 1188 to 1288) located at the KNT C terminus. The
region of the KNT protein that blocked phagosome transport (residues
295 to 612 and 568 to 943) and interacted with the inhibitory anti-KNT
antibody (residues 568 to 943) appears not to be involved in kinesin
binding. These conflicting results might be due to unspecific peptide
inhibition. Since the inhibitory KNT fragments form -helical coiled
coils, a common motif found in many proteins, these peptides may well
interfere with cellular processes other than KNT function. The anti-KNT
antibody does not necessarily need to bind directly to the KNT-kinesin
interaction domain to disrupt vesicle motility. The antibody could
interfere sterically with motor binding, provided that KNT is part of
or situated near a kinesin receptor complex on the vesicle membrane.
The removal of KNT from such a complex might still allow kinesin
binding to the organelle, whereas the addition of the antibody to the
complex does not.
The anterograde transport of lysosomes depends on kinesins (52), whereas the retrograde movement is mediated by cytoplasmic dynein (18). The overexpression of KNT-kinesin binding domains (KNT residues 1188 to 1288) suggested a function of KNT in anterograde lysosome trafficking (39). However, the requirement of KNT for lysosome transport could not be verified after the genetic inactivation of the knt gene (this study). Comparable to wild-type controls, anterograde lysosome transport does occur in the KNT-null mutant EF. Thus, it might be proposed that KNT does not play a role in lysosome motility or, alternatively, that KNT function is redundant and compensated for by hitherto-unidentified anchor proteins.
In summary, the role of KNT in kinesin-driven motility remains obscure. The functions of KNT, as suggested by various inhibition studies, could not be confirmed in a genetic approach by establishment of a KNT-defective mouse strain. Therefore, it must be determined whether KNT is merely part of a large multiprotein complex anchoring kinesin to the vesicle membrane but not essential for the interaction of the motor with the cargo. The analogy to the dynactin complex regulating cargo binding to the retrograde cytoplasmic dynein motors, as well as the recent reports of two distinct multiprotein anchors on vesicles for KIF13 and KIF17 may argue for this speculation (15, 24, 33, 48). However, the coupling of kinesin motors to vesicles need not be mediated by large multiprotein complexes. Very recently, APP and SYD (also known as JIP) have been described to bind directly to the TPR domain of the KLC (5, 26, 57). These transmembrane proteins could serve as cargo receptors for kinesin in fast axonal transport and post-Golgi transport, respectively. Whether KNT directly interacts with kinesin in vivo but is involved in the transport of a distinct class of vesicles rather than being an universal kinesin anchor remains to be determined. Alternatively, redundant family members might compensate for the KNT deficiency. Thus far, only one murine knt gene is known, and the search for homologues merely yielded one kinectin pseudogene (Plitz and Pfeffer, unpublished). However, the existence of a knt gene family cannot be ruled out. The KNT knockout mouse will provide a valuable tool to further analyze the biological significance of KNT.
| |
ACKNOWLEDGMENTS |
|---|
The continuous and generous support of H. Wagner is greatly appreciated. We thank M. Krönke for RS-TUM and the human knt cDNA, H. Häcker for GFPmut2, and B. Clausen for pBSlox-PneoloxP. We thank U. Huffstadt and E. Schaller for technical assistance and A. Fütterer, H. Flaswinkel, R. Endres, H. Häcker, and P. Ahmad-Nejad for scientific advice.
This work was supported by the Sonderforschungsbereich 391.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Institute of Medical Microbiology, Immunology & Hygiene, Technical University of Munich, Trogerstrasse 9, D-81675 Munich, Germany. Phone: 49-89-4140-4132. Fax: 49-89-4140-4139. E-mail: klaus.pfeffer{at}lrz.tum.de.
Present address: Serono Pharmaceutical Research Institute, CH-1228
Geneva, Switzerland.
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. |
Alimzhanov, M. B.,
D. V. Kuprash,
M. H. Kosco-Vilbois,
A. Luz,
R. L. Turetskaya,
A. Tarakhovsky,
K. Rajewsky,
S. A. Nedospasov, and K. Pfeffer.
1997.
Abnormal development of secondary lymphoid tissues in lymphotoxin beta-deficient mice.
Proc. Natl. Acad. Sci. USA
94:9302-9307 |
| 2. |
Ball, E. H., and S. J. Singer.
1982.
Mitochondria are associated with microtubules and not with intermediate filaments in cultured fibroblasts.
Proc. Natl. Acad. Sci. USA
79:123-126 |
| 3. |
Blocker, A.,
F. F. Severin,
J. K. Burkhardt,
J. B. Bingham,
H. Yu,
J. C. Olivo,
T. A. Schroer,
A. A. Hyman, and G. Griffiths.
1997.
Molecular requirements for bi-directional movement of phagosomes along microtubules.
J. Cell Biol.
137:113-129 |
| 4. |
Blose, S. H.,
D. I. Meltzer, and J. R. Feramisco.
1984.
10-nm filaments are induced to collapse in living cells microinjected with monoclonal and polyclonal antibodies against tubulin.
J. Cell Biol.
98:847-858 |
| 5. | Bowman, A. B., A. Kamal, B. W. Ritchings, A. V. Philp, M. McGrail, J. G. Gindhart, and L. S. Goldstein. 2000. Kinesin-dependent axonal transport is mediated by the Sunday driver (SYD) protein. Cell 103:583-594[CrossRef][Medline]. |
| 6. | Brady, S. T. 1985. A novel brain ATPase with properties expected for the fast axonal transport motor. Nature 317:73-75[CrossRef][Medline]. |
| 7. |
Chen, J. W.,
T. L. Murphy,
M. C. Willingham,
I. Pastan, and J. T. August.
1985.
Identification of two lysosomal membrane glycoproteins.
J. Cell Biol.
101:85-95 |
| 8. | Cormack, B. P., R. H. Valdivia, and S. Falkow. 1996. FACS-optimized mutants of the green fluorescent protein (GFP). Gene 173:33-38[CrossRef][Medline]. |
| 9. | Coy, D. L., W. O. Hancock, M. Wagenbach, and J. Howard. 1999. Kinesin's tail domain is an inhibitory regulator of the motor domain. Nat. Cell Biol. 1:288-292[CrossRef][Medline]. |
| 10. | Dabora, S. L., and M. P. Sheetz. 1988. The microtubule-dependent formation of a tubulovesicular network with characteristics of the ER from cultured cell extracts. Cell 54:27-35[CrossRef][Medline]. |
| 11. |
Desjardins, M.,
L. A. Huber,
R. G. Parton, and G. Griffiths.
1994.
Biogenesis of phagolysosomes proceeds through a sequential series of interactions with the endocytic apparatus.
J. Cell Biol.
124:677-688 |
| 12. | Friedman, D. S., and R. D. Vale. 1999. Single-molecule analysis of kinesin motility reveals regulation by the cargo-binding tail domain. Nat. Cell Biol. 1:293-297[CrossRef][Medline]. |
| 13. | Futterer, A., G. Kruppa, B. Kramer, H. Lemke, and M. Kronke. 1995. Molecular cloning and characterization of human kinectin. Mol. Biol. Cell 6:161-170[Abstract]. |
| 14. | Gepner, J., M. Li, S. Ludmann, C. Kortas, K. Boylan, S. J. Iyadurai, M. McGrail, and T. S. Hays. 1996. Cytoplasmic dynein function is essential in Drosophila melanogaster. Genetics 142:865-878[Abstract]. |
| 15. |
Gill, S. R.,
T. A. Schroer,
I. Szilak,
E. R. Stener,
M. P. Sheetz, and D. W. Cleveland.
1991.
Dynactin, a conserved, ubiquitously expressed component of an activator of vesicle motility mediated by cytoplasmic dynein.
J. Cell Biol.
115:1639-1650 |
| 16. | Goldstein, L. S., and A. V. Philp. 1999. The road less traveled: emerging principles of kinesin motor utilization. Annu. Rev. Cell Dev. Biol. 15:141-183[CrossRef][Medline]. |
| 17. | Gu, H., Y. R. Zou, and K. Rajewsky. 1993. Independent control of immunoglobulin switch recombination at individual switch regions evidenced through Cre-loxP-mediated gene targeting. Cell 73:1155-1164[CrossRef][Medline]. |
| 18. |
Harada, A.,
Y. Takei,
Y. Kanai,
Y. Tanaka,
S. Nonaka, and N. Hirokawa.
1998.
Golgi vesiculation and lysosome dispersion in cells lacking cytoplasmic dynein.
J. Cell Biol.
141:51-59 |
| 19. | Hentze, M. W., and A. E. Kulozik. 1999. A perfect message: RNA surveillance and nonsense-mediated decay. Cell 96:307-310[CrossRef][Medline]. |
| 20. |
Heuser, J.
1989.
Changes in lysosome shape and distribution correlated with changes in cytoplasmic pH.
J. Cell Biol.
108:855-864 |
| 21. |
Hirokawa, N.
1998.
Kinesin and dynein superfamily proteins and the mechanism of organelle transport.
Science
279:519-526 |
| 22. | Hirokawa, N., Y. Noda, and Y. Okada. 1998. Kinesin and dynein superfamily proteins in organelle transport and cell division. Curr. Opin. Cell Biol. 10:60-73[CrossRef][Medline]. |
| 23. | Hirokawa, N., K. K. Pfister, H. Yorifuji, M. C. Wagner, S. T. Brady, and G. S. Bloom. 1989. Submolecular domains of bovine brain kinesin identified by electron microscopy and monoclonal antibody decoration. Cell 56:867-878[CrossRef][Medline]. |
| 24. | Holleran, E. A., S. Karki, and E. L. Holzbaur. 1998. The role of the dynactin complex in intracellular motility. Int. Rev. Cytol. 182:69-109[Medline]. |
| 25. | Jahraus, A., B. Storrie, G. Griffiths, and M. Desjardins. 1994. Evidence for retrograde traffic between terminal lysosomes and the prelysosomal/late endosome compartment. J. Cell Sci. 107Pt 1:145-157[Abstract]. |
| 26. | Kamal, A., G. B. Stokin, Z. Yang, C. Xia, and L. S. Goldstein. 2000. Axonal transport of amyloid precursor protein is mediated by direct binding to the kinesin light chain subunit of kinesin-I. Neuron 28:449-459[CrossRef][Medline]. |
| 27. |
Kumar, J.,
H. P. Erickson, and M. P. Sheetz.
1998.
Ultrastructural and biochemical properties of the 120-kDa form of chick kinectin.
J. Biol. Chem.
273:31738-31743 |
| 28. |
Kumar, J.,
H. Yu, and M. P. Sheetz.
1995.
Kinectin, an essential anchor for kinesin-driven vesicle motility.
Science
267:1834-1837 |
| 29. |
Kuprash, D. V.,
M. B. Alimzhanov,
A. V. Tumanov,
A. O. Anderson,
K. Pfeffer, and S. A. Nedospasov.
1999.
TNF and lymphotoxin beta cooperate in the maintenance of secondary lymphoid tissue microarchitecture but not in the development of lymph nodes.
J. Immunol.
163:6575-6580 |
| 30. | Leung, E., C. G. Print, D. A. Parry, D. N. Closey, P. J. Lockhart, S. J. Skinner, D. C. Batchelor, and G. W. Krissansen. 1996. Cloning of novel kinectin splice variants with alternative C-termini: structure, distribution and evolution of mouse kinectin. Immunol. Cell Biol. 74:421-433[Medline]. |
| 31. |
Lippincott-Schwartz, J.,
N. B. Cole,
A. Marotta,
P. A. Conrad, and G. S. Bloom.
1995.
Kinesin is the motor for microtubule-mediated Golgi-to-ER membrane traffic.
J. Cell Biol.
128:293-306 |
| 32. | Machleidt, T., P. Geller, R. Schwandner, G. Scherer, and M. Kronke. 1998. Caspase 7-induced cleavage of kinectin in apoptotic cells. FEBS Lett. 436:51-54[CrossRef][Medline]. |
| 33. | Nakagawa, T., M. Seton, D. Seog, K. Ogasawara, N. Dohmae, K. Takio, and N. Hirokawa. 2000. A novel motor, KIF13A, transports mannose-6-phosphate receptor to plasma membrane through direct interaction with AP-1 complex. Cell 103:569-581[CrossRef][Medline]. |
| 34. |
Nakagawa, T.,
Y. Tanaka,
E. Matsuoka,
S. Kondo,
Y. Okada,
Y. Noda,
Y. Kanai, and N. Hirokawa.
1997.
Identification and classification of 16 new kinesin superfamily (KIF) proteins in mouse genome.
Proc. Natl. Acad. Sci. USA
94:9654-9659 |
| 35. |
Nakamura, N.,
C. Rabouille,
R. Watson,
T. Nilsson,
N. Hui,
P. Slusarewicz,
T. E. Kreis, and G. Warren.
1995.
Characterization of a cis-Golgi matrix protein, GM130.
J. Cell Biol.
131:1715-1726 |
| 36. |
Nakata, T., and N. Hirokawa.
1995.
Point mutation of adenosine triphosphate-binding motif generated rigor kinesin that selectively blocks anterograde lysosome membrane transport.
J. Cell Biol.
131:1039-1053 |
| 37. | Nangaku, M., R. Sato-Yoshitake, Y. Okada, Y. Noda, R. Takemura, H. Yamazaki, and N. Hirokawa. 1994. KIF1B, a novel microtubule plus end-directed monomeric motor protein for transport of mitochondria. Cell 79:1209-1220[CrossRef][Medline]. |
| 38. | Nonaka, S., Y. Tanaka, Y. Okada, S. Takeda, A. Harada, Y. Kanai, M. Kido, and N. Hirokawa. 1998. Randomization of left-right asymmetry due to loss of nodal cilia generating leftward flow of extraembryonic fluid in mice lacking KIF3B motor protein. Cell 95:829-837[CrossRef][Medline]. (Erratum, 99:117, 1999.) |
| 39. |
Ong, L. L.,
A. P. Lim,
C. P. Er,
S. Kuznetsov, and H. Yu.
2000.
Kinectin-kinesin binding domains and their effects on organelle motility.
J. Biol. Chem.
275:32854-32860 |
| 40. |
Ostwald, T. J., and D. H. MacLennan.
1974.
Isolation of a high affinity calcium-binding protein from sarcoplasmic reticulum.
J. Biol. Chem.
249:974-979 |
| 41. | Pfeffer, K., T. Matsuyama, T. M. Kundig, A. Wakeham, K. Kishihara, A. Shahinian, K. Wiegmann, P. S. Ohashi, M. Kronke, and T. W. Mak. 1993. Mice deficient for the 55 kd tumor necrosis factor receptor are resistant to endotoxic shock, yet succumb to L. monocytogenes infection. Cell 73:457-467[CrossRef][Medline]. |
| 42. | Plitz, T., U. Huffstadt, R. Endres, E. Schaller, T. W. Mak, H. Wagner, and K. Pfeffer. 1999. The resistance against Listeria monocytogenes and the formation of germinal centers depend on a functional death domain of the 55 kDa tumor necrosis factor receptor. Eur. J. Immunol. 29:581-591[CrossRef][Medline]. |
| 43. |
Rabinowitz, S.,
H. Horstmann,
S. Gordon, and G. Griffiths.
1992.
Immunocytochemical characterization of the endocytic and phagolysosomal compartments in peritoneal macrophages.
J. Cell Biol.
116:95-112 |
| 44. | Saxton, W. M., J. Hicks, L. S. Goldstein, and E. C. Raff. 1991. Kinesin heavy chain is essen-for viability and neuromuscular functions in Drosophila, but mutants show no defects in mitosis. Cell 64:1093-1102[CrossRef][Medline]. |
| 45. | Scholey, J. M., J. Heuser, J. T. Yang, and L. S. Goldstein. 1989. Identification of globular mechanochemical heads of kinesin. Nature 338:355-357[CrossRef][Medline]. |
| 46. | Schroer, T. A., and M. P. Sheetz. 1991. Functions of microtubule-based motors. Annu. Rev. Physiol 53:629-652[CrossRef][Medline]. |
| 47. |
Schwenk, F.,
U. Baron, and K. Rajewsky.
1995.
A cre-transgenic mouse strain for the ubiquitous deletion of loxP-flanked gene segments including deletion in germ cells.
Nucleic Acids Res.
23:5080-5081 |
| 48. |
Setou, M.,
T. Nakagawa,
D. H. Seog, and N. Hirokawa.
2000.
Kinesin superfamily motor protein KIF17 and mLin-10 in NMDA receptor-containing vesicle transport.
Science
288:1796-1802 |
| 49. |
Skouflas, D. A.,
D. G. Cole,
K. P. Wedaman, and J. M. Scholey.
1994.
The carboxyl-terminal domain of kinesin heavy chain is important for membrane binding.
J. Biol. Chem.
269:1477-1485 |
| 50. | Stenoien, D. L., and S. T. Brady. 1997. Immunochemical analysis of kinesin light chain function. Mol. Biol. Cell 8:675-689[Abstract]. |
| 51. |
Takeda, S.,
Y. Yonekawa,
Y. Tanaka,
Y. Okada,
S. Nonaka, and N. Hirokawa.
1999.
Left-right asymmetry and kinesin superfamily protein KIF3A: new insights in determination of laterality and mesoderm induction by kif3A/ mice analysis.
J. Cell Biol.
145:825-836 |
| 52. | Tanaka, Y., Y. Kanai, Y. Okada, S. Nonaka, S. Takeda, A. Harada, and N. Hirokawa. 1998. Targeted disruption of mouse conventional kinesin heavy chain, kif5B, results in abnormal perinuclear clustering of mitochondria. Cell 93:1147-1158[CrossRef][Medline]. |
| 53. |
Toyoshima, I.,
H. Yu,
E. R. Steuer, and M. P. Sheetz.
1992.
Kinectin, a major kinesin-binding protein on ER.
J. Cell Biol.
118:1121-1131 |
| 54. | Vale, R. D., and R. J. Fletterick. 1997. The design plan of kinesin motors. Annu. Rev. Cell Dev. Biol. 13:745-777[CrossRef][Medline]. |
| 55. |
Vale, R. D., and H. Hotani.
1988.
Formation of membrane networks in vitro by kinesin-driven microtubule movement.
J. Cell Biol.
107:2233-2241 |
| 56. | Vale, R. D., T. S. Reese, and M. P. Sheetz. 1985. Identification of a novel force-generating protein, kinesin, involved in microtubule-based motility. Cell 42:39-50[CrossRef][Medline]. |
| 57. |
Verhey, K. J.,
D. Meyer,
R. Deehan,
J. Blenis,
B. J. Schnapp,
T. A. Rapoport, and B. Margolis.
2001.
Cargo of kinesin identified as jip scaffolding proteins and associated signaling molecules.
J. Cell Biol.
152:959-970 |
| 58. | Whitaker, J. E., P. L. Moore, R. P. Haugland, and R. P. Haugland. 1991. Dihydrotetramethylrosamine: a long-wavelength, fluorogenic peroxidase substrate evaluated in vitro and in a model phagocyte. Biochem. Biophys. Res. Commun. 175:387-393[CrossRef][Medline]. |
| 59. | Yang, Z., D. W. Hanlon, J. R. Marszalek, and L. S. Goldstein. 1997. Identification, partial characterization, and genetic mapping of kinesin-like protein genes in mouse. Genomics 45:123-131[CrossRef][Medline]. |
| 60. |
Yonekawa, Y.,
A. Harada,
Y. Okada,
T. Funakoshi,
Y. Kanai,
Y. Takei,
S. Terada,
T. Noda, and N. Hirokawa.
1998.
Defect in synaptic vesicle precursor transport and neuronal cell death in KIF1A motor protein-deficient mice.
J. Cell Biol.
141:431-441 |
| 61. | Yu, H., C. V. Nicchitta, J. Kumar, M. Becker, I. Toyoshima, and M. P. Sheetz. 1995. Characterization of kinectin, a kinesin-binding protein: primary sequence and N-terminal topogenic signal analysis. Mol. Biol. Cell 6:171-183[Abstract]. |
Molecular and Cellular Biology, September 2001, p. 6044-6055, Vol. 21, No. 17
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.17.6044-6055.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
This article has been cited by other articles:
-
Hirokawa, N., Noda, Y.
(2008). Intracellular Transport and Kinesin Superfamily Proteins, KIFs: Structure, Function, and Dynamics. Physiol. Rev.
88: 1089-1118
[Abstract] [Full Text] -
Kamasani, U., Huang, M., DuHadaway, J. B., Prochownik, E. V., Donover, P. S., Prendergast, G. C.
(2004). Cyclin B1 Is a Critical Target of RhoB in the Cell Suicide Program Triggered by Farnesyl Transferase Inhibition. Cancer Res.
64: 8389-8396
[Abstract] [Full Text] -
Santama, N., Er, C. P. N., Ong, L.-L., Yu, H.
(2004). Distribution and functions of kinectin isoforms. J. Cell Sci.
117: 4537-4549
[Abstract] [Full Text] -
Palacios, I. M., Johnston, D. S.
(2002). Kinesin light chain-independent function of the Kinesin heavy chain in cytoplasmic streaming and posterior localisation in the Drosophila oocyte. Development
129: 5473-5485
[Abstract] [Full Text]
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
Copyright © 2009 by the American Society for Microbiology. For an alternate route to Journals.ASM.org, visit: http://intl-journals.asm.org | More Info»