From the Department of Medical Biochemistry,
University of Calgary, Calgary, Alberta T2N 4N1, Canada and
¶ Department of Biochemistry, Hong Kong University of
Science and Technology, Clear Water Bay, Kowloon, Hong Kong
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ABSTRACT |
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Cdk5 exists in brain extracts in multiple forms, one of which is a macromolecular protein complex comprising Cdk5, neuron-specific Cdk5 activator p35nck5a and other protein components (Lee, K.-Y., Rosales, J. L., Tang, D., and Wang, J. H. (1996) J. Biol. Chem. 271, 1538-1543). The yeast two-hybrid system was employed to identify p35nck5a-interacting proteins from a human brain cDNA library. One of the isolated clones encodes a fragment of glial fibrillary acidic protein, which is a glial-specific protein. Sequence alignment revealed significant homology between the p35nck5a-binding fragment of glial fibrillary acidic protein and corresponding regions in neurofilaments. The association between p35nck5a and neurofilament medium molecular weight subunit (NF-M) was confirmed by both the yeast two-hybrid assay and direct binding of the bacteria-expressed proteins. The p35nck5a binding site on NF-M was mapped to a carboxyl-terminal region of the rod domain, in close proximity to the putative Cdk5 phosphorylation sites in NF-M. A region immediately amino-terminal to the kinase-activating domain in p35nck5a is required for its binding with NF-M. In in vitro binding assays, NF-M binds both monomeric p35nck5a and the Cdk5/p35nck5a complex. The binding of NF-M has no effect on the kinase activity of Cdk5/p35nck5a.
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INTRODUCTION |
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Neuronal Cdc2-like kinase (Nclk)1 was originally purified from bovine brains on the basis of its phosphorylating activity toward serine or threonine within the sequence motif Ser/Thr-Pro-X-Lys/Arg (X for any amino acid) (1). In an independent study, Nclk was also isolated as a tau protein kinase since it catalyzed in vitro phosphorylation of tau, which is a brain microtubule-associated protein (2, 3). Purified Nclk is a heterodimer of Cdk5 and a 25-kDa regulatory subunit (p25), which is derived proteolytically from a brain and neuron-specific 35-kDa protein (p35) (4-6). In view of its specific Cdk5 activating activity, p25/p35 is called neuronal Cdk5 activator (Nck5a). In addition, mammalian brains also contain a neuron-specific 39-kDa isoform of Nck5a, called neuronal Cdk5 activator isoform (Nck5ai) (7). Nck5a and Nck5ai display a high degree of protein sequence identity, but share little sequence homology with members of the cyclin family, thus suggesting that they represent a novel family of Cdk-activating proteins.
Along with its unique structure, Nck5a is endowed with unique regulatory properties distinct from those of cyclins. While the activation of Cdc2 by cyclin depends on phosphorylation of Cdc2 by a Cdk-activating kinase at a specific threonine residue (Thr-161), the activation of Cdk5 by Nck5a is independent of Cdk5 phosphorylation (8-11). Also, several Cdc2-like kinases have been shown to be inactivated readily upon tyrosine phosphorylation by a Wee1 kinase (8, 9). However, Cdk5/Nck5a is only sluggishly phosphorylated and inactivated by Wee1 (12, 13). In addition, Cdk-cyclin complexes are susceptible to inhibitory activities of specific inhibitory proteins, such as p21cip1/WAF1 and p27kip1 (8, 9, 14). In contrast, the kinase activity of Nclk is resistant to these proteins (15, 16).
Developmental, cell biological, and transgenic mouse studies have implicated Nclk as an important regulator in development of the central nervous system in mammals and in normal functions of terminally differentiated neurons (5-7, 17-23). The apparent involvement of Nclk in neuronal differentiation and brain functions may be attributed to the roles of this enzyme in neurocytoskeletal dynamics. Among in vitro Nclk substrates are neuron-specific cytoskeletal proteins such as tau and neurofilaments (3, 24-27). In Alzheimer patients, tau from neurofibrillary tangles is hyperphosphorylated on many proline-directed Ser/Thr sites (28). A number of studies have suggested that Nclk is a major kinase involved in catalyzing the proline-directed tau phosphorylation (2, 29). Mammalian neurofilaments consist of three protein components, neurofilament high (NF-H), medium (NF-M), and low (NF-L) molecular weight subunits, which are assembled into neurofilaments and transported down axons as discrete cytological structures (30-32). During this transport, NF-H and NF-M are heavily phosphorylated on their tail domains at many proline-directed Ser/Thr sites (33, 34). Cdk5 has been suggested to participate in this axonal transport-dependent phosphorylation of the neurofilament proteins (24-27). This suggestion is supported by the observation that, in cultured neuronal cells, both Cdk5 and Nck5a are present throughout the axons where neurofilaments represent the bulk of the cytoskeletal proteins (18). In the present study, we show that Nck5a and Nclk associate specifically with the neurofilament proteins, an observation that may be the molecular basis of the colocalization and possible co-transportation of Nclk and neurofilaments in the axons. Our characterization of the interaction between Nck5a and neurofilaments is compatible with the notion that, in addition to kinase activation, Nck5a functions in anchoring Cdk5 to its kinase substrates.
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EXPERIMENTAL PROCEDURES |
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Library Screening with the Yeast Two-hybrid System--
The
bovine p35nck5a-coding sequence was amplified by PCR with the
primers of NCK-1 (5-CCAGCCATGGGCACGGTGCTGTCC-3
) and NCK-2
(5
-CTGGGATCCTCACCGGTCCAGCCCGAG-3
). The PCR fragment was inserted into
the GAL4 DNA binding domain plasmid pAS2 at NcoI
and BamHI, resulting in a bait plasmid
p35nck5a/pAS2. The prey is a human brain
cDNA library in the GAL4 transcription activation domain plasmid
pACT2 (CLONTECH Laboratories, Inc.). The
bait and prey were sequentially transformed into yeast
CG-1945 (MATa, ura3-52, his3-200,
lys2-801, trp1-901, ade2-101, leu2-3, 112, gal4-542, gal80-538,
LYS2::GAL1-HIS3, cyhr2,
URA3::(GAL4 17-mers)3-CYC1-lacZ). The
cotransformants harboring two interacting proteins were selected on a
synthetic dextrose medium lacking leucine, tryptophan, and histidine,
but including 5 mM 3-amino-1,2,4-triazole, and tested for
-galactosidase activity by a filter lift assay with X-gal (35).
Primary positive clones were recovered and then transformed into yeast
Y190 (MATa, leu2-3, 112, ura3-52,
trp1-901, his3-
200, ade2-101, gal4
gal80
URA3 GAL-lacZ, LYS
GAL-HIS3, cyhr) with
p35nck5a/pAS2, pAS2, and
lamin C/pAS (a fragment of human lamin C engineered in frame
in pAS) individually (36). The library plasmids that activated the reporter transcription only in the presence of
p35nck5a/pAS2 were considered as positive
clones and analyzed further.
Cloning of Nck5a and NF-M Fragments--
pAS2
constructs containing truncated fragments of bovine p35nck5a
were generated following the PCR strategy. p351-98 was
amplified with the primers of NCK-1 and NCK-3
(5-CCGGATCCGAACGTGGACAGGTTGGC-3
). The
NH2-terminal-deleted fragments of Nck5a were achieved with the antisense primer NCK-2 and different sense primers: NCK-4 (5
-CAGCCATGGCCCAGCCCCCGCCGGCC-3
) for p3599-307, NCK-5
(5
-CGACCATGGCCCCCCCTGCCAGCCAG-3
) for p35108-307, NCK-6
(5
-CGACCATGGTCCAGGCGTCCACCAGC-3
) for p35144-307, NCK-7
(5
-CGACCATGGAGCTGCTGCGCTGCCTG-3
) for p35150-307.
They were inserted into pAS2 at NcoI and
BamHI sites. p39nck5ai/pAS2
has the coding sequence of Nck5ai cloned in frame in the DNA binding
domain vector.
Preparation of Fusion Proteins--
GST fusion proteins were
expressed in bacteria and purified following the procedure described
previously (10). p35nck5a was expressed in Escherichia
coli strain M15(pREP4) transformed with
p35nck5a/pQE12. The expressed protein has
a hexahistidine tag COOH-terminal to p35nck5a
(p35nck5a-His). For isolation of p35nck5a-His, cells
were lysed in lysis buffer (10 mM Tris-HCl, pH 8.0, 0.5 M NaCl, 1% Triton X-100, 10 mM imidazole, 10 mM -mercaptoethanol, 0.5 mM PMSF, 10 mM benzamidine, 1 µg/ml each of leupeptin, aprotinin, and
antipain) by passing the cell suspension through a French Press machine
(1000 p.s.i.). After clarification of the cell lysate by
centrifugation, the supernatant was loaded on Ni-nitriloacetic acid-agarose (Qiagen). The beads were then sequentially washed in a
column with buffer A (10 mM Tris-HCl, pH 7.5, 1 M NaCl, 25 mM imidazole, 0.5% Triton X-100, 10 mM
-mercaptoethanol, 3 mM benzamidine, and
0.5 mM PMSF), and buffer B (10 mM Tris-HCl, pH 7.5, 0.15 M NaCl, 5 mM imidazole, 6 mM
-mercaptoethanol, 3 mM benzamidine, and
0.5 mM PMSF). The bound protein was eluted with 10 mM Tris-HCl, pH 7.5, 0.15 M NaCl, 350 mM imidazole, 6 mM
-mercaptoethanol, 3 mM benzamidine, and 0.5 mM PMSF. The eluate was
dialyzed against 10 mM Tris-HCl, pH 7.5, 20 mM
NaCl, 1 mM EDTA and 1 mM dithiothreitol.
In Vitro Binding Assays-- GST or GST-NF-M fragments were mixed with p35-His or the Cdk5/p25nck5a complex in a 50-µl volume and incubated at 30 °C for 30 min. After addition of 100 µl of bead slurries containing approximately 20 µl of GSH-Sepharose 4B (Pharmacia Biotech Inc.) in washing buffer (25 mM Tris-HCl, pH 7.5, 50 mM NaCl, 0.1% Triton X-100, 1 mM EDTA, 1 mM dithiothreitol, and 0.2 mM PMSF), the incubation was continued with shaking for 1 h at 4 °C. The Sepharose beads were then collected and washed extensively with the washing buffer. Bound proteins were dissolved in SDS-PAGE sample buffer and subjected to SDS-PAGE. Alternatively, the bound proteins were eluted with GSH buffer (25 mM Tris-HCl, pH 7.5, 50 mM NaCl, 1 mM dithiothreitol, and 20 mM GSH), and subjected to protein phosphorylation reactions.
Protein Phosphorylation Reactions--
The Cdk5 kinase activity
was measured by phosphorylation of the histone H1 peptide HS(9-18) as
described previously (10). Phosphorylation of NF-M fragments was
carried out at 30 °C in a mixture containing 20 mM MOPS
at pH 7.5, 5 mM MgCl2, 100 µM [-32P]ATP (~5000 dpm/pmol), 1 mM
dithiothreitol, and indicated protein samples. The reactions were
terminated by addition of SDS-PAGE sample buffer. The samples were
boiled for 5 min before loading on gels. Protein phosphorylation was
visualized by autoradiography.
SDS-PAGE and Immunoblots-- SDS-PAGE was performed by the method of Laemmli in vertical slab gels (37). For immunoblots, proteins were resolved by SDS-PAGE, transferred to Immobilon polyvinylidene difluoride membrane (Millipore), and probed with particular antibodies as indicated. Blots were visualized by enhanced chemiluminescence according to the manufacturer's procedure (Amersham Life Science, Inc.). The antibodies recognizing Cdk5 and Nck5a are monoclonal and polyclonal antibody preparations, respectively, generated in our laboratory.
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RESULTS |
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In a previous study, we showed that Nck5a existed in bovine brain extracts either as a 25-kDa fragment in a heterodimeric complex of Cdk5/p25nck5a, or as the full-length protein (p35nck5a) in a macromolecular complex of over 600 kDa, which also contained Cdk5 as a constituent protein (38). This observation has led to the suggestion that p35nck5a has the ability to undergo high affinity association with certain cellular proteins. The yeast two-hybrid system was therefore employed to screen a human brain cDNA library to identify the putative p35nck5a-binding proteins. About 3.5 × 105 cotransformants were analyzed. A total of 108 positive clones were isolated and introduced into another yeast strain to test binding specificities. 14 clones from the primary isolates displayed specific interaction with the original bait p35nck5a/pAS2. Upon sequence analysis, these 14 clones were revealed to originate from seven different cDNA sequences. One of the isolated sequences, which represents three individual clones, encodes a carboxyl-terminal fragment of glial fibrillary acidic protein (GFAP).
Since Nck5a is a neuron-specific protein, whereas the expression of GFAP is restricted to glial cells, it is unlikely that these two proteins associate in brains under normal physiological conditions. However, the association of Nck5a with GFAP may reflect the ability of Nck5a to undergo association with certain neuronal proteins containing protein sequences similar to that of the Nck5a-binding region of GFAP. GFAP is a member of the intermediate filament family (30). All intermediate filaments share the basic architecture of a conserved central rod domain flanked by variable head and tail domains (30). The isolated Nck5a-binding fragment consists of a carboxyl-terminal portion of the rod domain and the entire tail region of GFAP. Among the intermediate filament family members are the neuron-specific intermediate filaments, NF-L, NF-M and NF-H (30-32). NF-M and NF-H have been suggested as in vivo substrates of Cdk5 (3, 24-27). Sequence alignment displays high degrees of protein sequence identity between the Nck5a-binding region of GFAP and the corresponding rod regions in neurofilaments (Fig. 1), suggesting that Nck5a may bind neurofilaments in cells.
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To test whether neurofilaments are indeed capable of association with Nck5a, a fragment of NF-M, NF-M346-467, corresponding to the Nck5a-binding fragment of GFAP, was engineered into the plasmid pACT2 for the two-hybrid assay. As shown in Fig. 2, the reporter activity was detected when NF-M346-467/pACT2 was cotransformed with p35nck5a/pAS2 into yeast cells, whereas cotransformation of a control plasmid lamin C/pAS2 with the NF-M346-467/pACT2 displayed no reporter activity. The result suggests that NF-M could indeed associate with Nck5a in the yeast. The fragment NF-M346-467 is composed of a carboxyl-terminal region of the conserved core domain and an amino-terminal region of the tail domain of NF-M. To localize more precisely the p35nck5a-binding region in NF-M, the pACT2 constructs of NF-M346-413 and NF-M411-467 were generated, corresponding to the rod domain and the tail domain fragments, respectively. As shown in Fig. 2, cotransformation of the rod domain fragment (NF-M346-413) with Nck5a strongly activated the reporter activity, whereas no detectable reporter activity appeared in the cotransformants of the tail fragment construct NF-M411-467/pACT2 and p35nck5a/pAS2. This observation indicates that the carboxyl-terminal portion of the NF-M rod domain, which is no more than 16% of the rod domain, is sufficient for the binding with Nck5a, and the tail region is not required for this interaction. Since Cdk5 phosphorylation sites in NF-M and NF-H are located at the carboxyl-terminal tails, the localization of the Nck5a-binding site immediately amino-terminal to the tail region may be significant for the kinase reaction. Mammalian brains contain an isoform of Nck5a, p39nck5i (7). Fig. 3 shows that p39nck5i did not give rise to positive response when tested for its ability to bind NF-M using the yeast two-hybrid system. The result demonstrates specificity of the interaction between Nck5a and NF-M.
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Nck5a exists in bovine brain extracts either as a full-length protein of 307 amino acids or an amino-terminal-truncated form (p25nck5a), which consists of residues 99-307 of p35nck5a (38). To determine whether the interaction between NF-M and Nck5a requires the amino-terminal region of Nck5a, we dissected p35nck5a into two fragments: the amino-terminal fragment (p351-98) and the fragment of p25nck5a (p3599-307). These two fragments as well as the full-length Nck5a were tested for their abilities to bind NF-M in the yeast two-hybrid system. Figs. 2 and 3 show that NF-M interacts with both full-length Nck5a and p25nck5a, but not with the amino-terminal fragment (p351-98). This observation suggests that the NF-M binding site is located within residues 99-307 of Nck5a. To define more precisely the region required for the NF-M binding, various amino-terminal-truncated forms of Nck5a were constructed and tested for their interactions with NF-M by the yeast two-hybrid assay. The results were summarized in Fig. 4. It indicates that a short stretch of protein sequence spanning residues 144 to 150 is required for the NF-M binding. Recently, the Cdk5-activating domain in Nck5a has been mapped to a region of amino acid residues 150-291 (12, 39). It should be noted that the region immediately amino-terminal to the minimal Cdk5-activating domain in Nck5a is essential for its interaction with NF-M.
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To provide direct proof for the specific association between NF-M and Nck5a, this protein-protein interaction was carried out and characterized in vitro using bacterially expressed proteins. GST-fusion proteins of two NF-M carboxyl-terminal fragments: NF-M346-915 and NF-M411-915, were expressed in and isolated from bacteria (Figs. 5, A and B). The results from the yeast two-hybrid assay suggested that NF-M346-915 contains the Nck5a-binding site, whereas NF-M411-915 does not. To demonstrate protein associations, the GST-NF-M proteins were incubated with (His)6-tagged p35nck5a and then affinity-precipitated using GSH beads. The precipitates were then analyzed on an immunoblot using an anti-Nck5a antibody to determine whether Nck5a had co-precipitated with the NF-M fragments. Fig. 5C shows that the bacteria-expressed and affinity-purified p35nck5a-His contains intact p35nck5a and two partially proteolyzed fragments showing immunoreactive protein bands of approximately 30 and 28 kDa. The p35nck5a-His proteins were present in the precipitate of GST-NF-M346-915 but not in the precipitates of GST and GST-NF-M411-915 (Fig. 5C). It supports the results from the yeast two-hybrid analysis suggesting that Nck5a undergoes specific association with NF-M and that the Nck5a-binding site is localized at the carboxyl-terminal region of the NF-M rod domain.
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To further characterize the interaction between NF-M and Nck5a, the interaction was examined with the heterodimer of Cdk5/p25nck5a, which is the active form of Nclk existing in bovine brain extracts. Nclk was prepared by reconstitution from bacterially expressed Cdk5 and p25nck5a as described previously (10). Samples of Nclk were incubated with GST-NF-M346-915, GST-NF-M411-915, and GST separately. The GST fusion proteins were then affinity-precipitated using GSH beads. After being washed extensively, the precipitates were subjected to immunoblot analysis using antibodies against Cdk5 and Nck5a. As shown in Fig. 6, both Cdk5 and Nck5a could be detected in the precipitated sample containing GST-NF-M346-915 but not in those of GST-NF-M411-915 and GST. The binding of Nclk and NF-M346-915 is essentially quantitative under the experimental conditions. The results indicate that NF-M binds both Nck5a monomer and the Cdk5/Nck5a heterodimer, and the same site in NF-M may be involved in the binding of the two protein species.
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To further address the question of potential physiological significance of the interaction between NF-M and Nck5a, we examined any effect on the Cdk5-activating activity of Nck5a by interaction with NF-M. In one experiment, the activation of Cdk5 by a suboptimal amount of p25nck5a was determined in the presence of NF-M346-915. It was found that NF-M346-915, over a large concentration range, could neither enhance nor impede the Cdk5-activating activity of Nck5a (Fig. 7A). All three proteins used in the experiment of Fig. 7A were bacterially expressed GST fusion proteins. However, similar results were obtained if the proteins were pretreated by thrombin to remove the GST moiety (data not shown). To ensure that the kinase activity measured was indeed that of NF-M-bound Nclk, samples of reconstituted Cdk5/p25nck5a were incubated with varying amounts of GST-NF-M346-915. GST-NF-M346-915 along with its bound-Nclk was then affinity-precipitated using GSH beads and the Cdk5 kinase activity in the precipitates was then assayed. As shown in Fig. 7B, the Cdk5 kinase activity could be recovered in the precipitates in a NF-M346-915 concentration-dependent manner. The kinase in the precipitate could also phosphorylate NF-M as shown in Fig. 7C. In a separate experiment, the Cdk5-catalyzed phosphorylation of NF-M346-915 was compared with that of NF-M411-915, and they were about the same (data not shown). NF-M346-915 is capable of binding to Nck5a, but NF-M411-915 is not. Thus, under various conditions, NF-M-bound Nclk and free Nclk appeared to have the same kinase activity.
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DISCUSSION |
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It has become increasingly clear that protein-protein interactions
play key roles in cellular regulatory mechanisms. The present study
shows that neurofilament NF-M undergoes a specific association with
Nck5a. The region of NF-M involved in the Nck5a binding is conserved in
NF-H and NF-L, suggesting that these neurofilament proteins are also
capable of associating with Nck5a. Several lines of evidence implicate
that NF-M and NF-H are in vivo substrates of Nclk. For
example, NF-M and NF-H are heavily phosphorylated in neurons on their
carboxyl-terminal regions at proline-directed Ser/Thr residues. Many of
these in vivo phosphorylation sites can be phosphorylated
in vitro by reconstituted reactions containing purified and
dephosphorylated neurofilament proteins and Nclk (3, 24, 25).
Cotransfection of SW13cl2Vim cells, which are lacking
cytoplasmic intermediate filaments, with Cdk5, Nck5a, and NF-H
generated heavily phosphorylated NF-H in the cells, whereas
transfection of NF-H with Cdk5, Nck5a, and a dominant negative mutant
of Cdk5 failed to phosphorylate NF-H (25). glycogen synthase kinase
3
is another proline-directed Ser/Thr protein kinase that has been
suggested to catalyze tau phosphorylation in brains (40). When NF-H was
introduced into SW13cl2Vim
cells with glycogen synthase
kinase 3
, there was no significant extent of NF-H phosphorylation
observed (25). The interaction between Nck5a and the NF subunits
suggests that Nck5a, in addition to being an activator of Cdk5, serves
as an anchoring protein to localize Cdk5 to its protein substrates.
This may provide a molecular mechanism for the colocalization of
neurofilaments and Nclk.
While the use of anchoring proteins to localize an enzyme to its specific site of action may no longer be considered as a novel observation, the highly asymmetrical morphology of neurons and the unique distribution and movement of neurofilaments in neurons have rendered the need for such an anchoring function in the neurofilament phosphorylation system especially obvious and important. Neurofilament proteins are synthesized in the neuronal cell body and assembled at the entrance of the axon. Immediately after the assembly, neurofilaments are transported toward the distal region of the axon along with other cytoskeletal proteins as a discrete structure. It is during this axonal transport, that the carboxyl-terminal tails of NF-H and NF-M become phosphorylated. Both Cdk5 and Nck5a are present in and throughout the axon in cultured mammalian embryonic neurons (18). The interaction between Nck5a and neurofilaments appears to be the molecular basis of the axonal localization of Nck5a and Cdk5. Furthermore, the association of Nclk to neurofilaments suggests that Nclk may be transported together with neurofilaments in the axon.
Several features of the interaction between Nck5a and neurofilaments are compatible with such a suggestion. The binding of NF-M to Nck5a is localized proximal to the amino-terminal junction of the Cdk5-activating domain of Nck5a. As a result, the binding of NF-M has no effect on the Cdk5-activating activity of Nck5a. In addition, the Nck5a-binding site on NF-M borders on the amino terminus of the tail region where the putative Cdk5 phosphorylation sites are located. It seems to be strategically localized to maximize the Cdk5 activity as a neurofilament kinase. Indeed, the phosphorylation of NF-M by NF-M-bound Nclk has been demonstrated in the present study.
While significant advances have been made in elucidation of the general regulatory properties of the Cdk family, the regulation of Cdk5 appears to be governed by distinct mechanisms which are poorly understood. Cdk5 activation by Nck5a does not require Cdk-activating kinase and Cdk5 is not phosphorylated in highly active Nclk (10). Also, Cdk5/Nck5a shows significant resistance to the Wee1 kinase and p21cip1/WAF1 and p27kip1, which are common Cdk inhibitory kinase and inhibitory proteins, respectively (12, 13, 15, 16). On the other hand, phosphorylation of the neurofilament proteins during axonal transport is temporally regulated, since the extent of the protein phosphorylation increases gradually during the transport. Knowledge of how the neurofilament kinase is regulated in this process awaits elucidation of the regulatory properties of Cdk5 and Nclk. Perhaps some of the other Nck5a-binding proteins identified by the two-hybrid screening procedure are factors that can regulate Nclk. Most of the Cdk5 protein in bovine brain extracts exists in an inactive state either as monomeric Cdk5 or as a macromolecular complex that also contains the full-length Nck5a (38). Circumstantial evidence in the literature points to the existence in mammalian brains of a inhibitory protein factor(s) and a inhibitory protein kinase(s) for Cdk5 (38, 41).
Protein-protein interactions detected in the yeast two-hybrid system do not necessarily mean that the interactions occur in vivo. However, even a nonphysiological interaction may provide insight into physiologically relevant reactions. The initial interaction detected in this study was between Nck5a and a glial-specific protein GFAP, and neurofilaments were not in the isolated seven sequences encoding p35nck5a-binding proteins. The distinct localizations of GFAP and Nck5a in brains have ruled out this protein-protein association as being physiologically significant. However, this interaction has led to the identification of closely related NF-M as a Nck5a-binding protein. The interaction between Nck5a and neurofilaments has obvious physiological significance. Elucidation of the molecular basis of this protein-protein interaction may shed important light on the mechanism of Nclk action and function in neurons.
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ACKNOWLEDGEMENTS |
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We thank Dr. C. J. Brandl (University of Western Ontario) for his valuable advice and help with the yeast two-hybrid system. We are also grateful to Dr. M. Treuner for discussion throughout the work and reading the manuscript, and F. Hwang for technical assistance.
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FOOTNOTES |
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* This work was supported in part by operating grants from the Medical Research Council of Canada and the Research Grant Council of the Hong Kong Government, and an group grant from the Alberta Cancer Board (Canada).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
§ Recipient of the Alberta Cancer Board Postdoctoral Fellowship.
Scientist of the Alberta Heritage Foundation for Medical
Research.
** Recipient of the Alberta Heritage Foundation for Medical Research travel award. To whom correspondence should be addressed: Dept. of Biochemistry, Hong Kong University of Science and Technology, Clear Water Bay, Kowloon, Hong Kong. Tel.: 852-2358-8701; Fax: 852-2358-2765; E-mail: jerwang{at}usthk.ust.hk.
1
The abbreviations used are: Nclk, neuronal
Cdc2-like kinase; Nck5a, neuronal Cdk5 activator; Nck5ai, neuronal Cdk5
activator isoform; NF-H, -M, and -H, neurofilament high, medium, and
low molecular weight subunits; GST, glutathione
S-transferase; MOPS, 4-morpholinepropanesulfonic acid; PAGE,
polyacrylamide gel electrophoresis; PCR, polymerase chain reaction;
PMSF, phenylmethylsulfonyl fluoride; X-gal,
5-bromo-4-chloro-3-indolyl--D-galactopyranoside; GFAP, glial fibrillary acidic protein.
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REFERENCES |
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