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© The Rockefeller University Press, 0021-9525/1999//377 $5.00
The Journal of Cell Biology, Volume 145, Number 2, , 1999 377-389

Dual Fatty Acylation of p59^Fyn Is Required for Association with the T Cell Receptor Chain through Phosphotyrosine–Src Homology Domain-2 Interactions

Cell Biology Program, Memorial Sloan-Kettering Cancer Center, New York 10021

The first 10 residues within the Src homology domain (SH)–4 domain of the Src family kinase Fyn are required for binding to the immune receptor tyrosine-based activation motif (ITAM) of T cell receptor (TCR) subunits. Recently, mutation of glycine 2, cysteine 3, and lysines 7 and 9 was shown to block binding of Fyn to TCR chain ITAMs, prompting the designation of these residues as an ITAM recognition motif (Gauen, L.K.T., M.E. Linder, and A.S. Shaw. 1996. J. Cell Biol. 133:1007–1015). Here we show that these residues do not mediate direct interactions with TCR ITAMs, but rather are required for efficient myristoylation and palmitoylation of Fyn. Specifically, coexpression of a K_7,9A-Fyn mutant with N-myristoyltransferase restored myristoylation, membrane binding, and association with the cytoplasmic tail of TCR fused to CD8. Conversely, treatment of cells with 2-hydroxymyristate, a myristoylation inhibitor, blocked association of wild-type Fyn with . The Fyn NH₂ terminus was necessary but not sufficient for interaction with and both Fyn kinase and SH2 domains were required, directing phosphorylation of ITAM tyrosines and binding to ITAM phosphotyrosines. Fyn/ interaction was sensitive to octylglucoside and filipin, agents that disrupt membrane rafts. Moreover, a plasma membrane bound, farnesylated Fyn construct, G₂A,C₃S-FynKRas, was not enriched in the detergent insoluble fraction and did not associate with . We conclude that the Fyn SH4 domain provides the signals for fatty acylation and specific plasma membrane localization, stabilizing the interactions between the Fyn SH2 domain and phosphotyrosines in TCR chain ITAMs.

Key Words: Src homology domains • acylation • cell membrane • protein-tyrosine kinase • receptor/ antigen

Abbreviations used in this paper: GFP, green fluorescent protein; ITAM, immune-receptor tyrosine-based activation motif; NMT, N-myristoyl transferase; SH, Src homology domain; TCR, T cell receptor.

Address correspondence to Marilyn D. Resh, Cell Biology Program, Memorial Sloan-Kettering Cancer Center, 1275 York Ave., Box 143, New York, NY 10021. Tel.: (212) 639-2514. Fax: (212) 717-3317. E-mail: m-resh{at}ski.mskcc.org

PROTEINS belonging to the Src family of nonreceptor tyrosine kinases critically rely on binding to the cytoplasmic leaflet of the plasma membrane lipid bilayer to fulfill their biological functions (32, 40). Membrane targeting is specifically guided by the Src homology domain (SH)¹–4 motif, a short sequence in the NH₂-terminal region of Src family kinases (30, 31). SH4 motifs contain two independent signals (myristate and either palmitate or a polybasic amino acid sequence) that control stable membrane attachment when acting together, but not when operating individually (31, 32). For example, specific and rapid plasma membrane targeting of the Src family kinase Fyn is encoded by dual fatty acylation with myristate at glycine 2 and palmitate at cysteine 3 (1, 35, 41, 43).

Protein myristoylation involves the cotranslational attachment of the 14 carbon fatty acid myristate to the NH₂-terminal glycine (glycine 2) on target proteins (8, 17, 42). A chemically stable amide bond is formed between myristate and glycine and is maintained for the lifetime of the protein. The enzymatic reaction is catalyzed by N-myristoyl transferase (NMT), a cytosolic protein that is ubiquitously expressed in eukaryotic cells. The minimum consensus sequence for N-myristoylation is GXXXS/T; glycine 2 is a critical component and a serine or threonine at position 6 is preferred (17). Additional amino acids have been shown to be important for recognition by NMT in the context of specific protein sequences. N-myristoylation of Fyn is a prerequisite for posttranslational and dynamic palmitoylation to occur. Mutations that ablate myristoylation result in loss of palmitoylation (1, 35, 41, 43). Efficient myristoylation of Fyn, therefore, is essential for correct processing and intracellular targeting of Fyn (41, 43).

One of the functional consequences of dual fatty acylation and plasma membrane targeting is to allow Src family kinases to interact with transmembrane receptor complexes. For example, Fyn coimmunoprecipitates with the activated T cell receptor (TCR) and has been reported to interact with multiple TCR subunits (10, 33). Fyn tyrosine kinase activity is stimulated when the TCR is cross-linked, but the molecular nature of the Fyn/TCR interaction is not entirely clear, as the complex is only detected by the use of mild detergents to lyse cells (10, 33, 40). The presence of immune receptor tyrosine-based activation motifs (ITAM) on the chain of the TCR was shown to be essential for interaction with Fyn, although no specific amino acid within the ITAM seemed to be responsible for this interaction (12). Recently, mutation of glycine 2, cysteine 3, and lysines 7 and 9 within the SH4 domain of Fyn was reported to block binding to the chain of the TCR, prompting the designation of these four resides as an ITAM recognition motif (11). However, glycine 2 is required for myristoylation and cysteine 3 is the main site of palmitoylation in Fyn (1, 35, 43). In addition, lysine 7 has been implicated in directing efficient myristoylation of Src (6, 19). Thus, it remained possible that alteration in fatty acylation levels was responsible for the inability of the mutant Fyn to interact with chain.

We therefore reevaluated the role of the SH4 motif of Fyn, focusing on the significance of lysines 7 and 9 in fatty acylation and membrane targeting of Fyn, and its interactions with the TCR chain. Here we show that dual fatty acylation of a K_7,9A-Fyn mutant was drastically impaired. A gain of function experiment revealed that overexpression of NMT restored fatty acylation levels of K_7,9A-Fyn and allowed the mutant protein to interact with the cytoplasmic tail of the TCR chain fused to CD8. Using the myristoylation inhibitor 2-hydroxymyristate, we observed that association of wild-type Fyn with the chain can be disrupted by blocking fatty acylation. The Fyn NH₂ terminus was necessary but not sufficient for interaction with . Both functional Fyn kinase and SH2 domains were required, directing phosphorylation of ITAM tyrosines and subsequent binding of the Fyn SH2 domain to ITAM phosphotyrosines. The interactions between Fyn and were sensitive to conditions that disrupt membrane rafts and a farnesylated Fyn construct that was not enriched in the detergent insoluble fraction did not stably associate with .

These results provide additional explanations for the sequence requirements and mild detergent conditions needed for coimmunoprecipitation of Fyn with TCR subunits. We conclude that dually fatty acylation of Fyn is required for correct targeting to specific membrane subdomains, that is a prerequisite for stable association with the cytoplasmic tail of the TCR chain. Fyn kinase activity is required for phosphorylation of tyrosine residues in the ITAMs of the chain, to which the Fyn SH2 domain subsequently binds. The localization of Fyn in plasma membrane rafts therefore serves an essential role in stabilizing SH2–phosphotyrosine interactions between Fyn and TCR .

	Materials and Methods

Top Abstract Materials and Methods Results Discussion References

 
Materials
Cell culture reagents were purchased from Gibco Laboratories. cDNAs for human wild-type Fyn, G₂A-Fyn, and C_3,6S-Fyn (1) and NMT (28) and rabbit polyclonal antiserum raised against Fyn SH43 protein (3) were from lab stocks. pEFBOS-CD8-, CD8-T76, and CD8-4F (16, 22) were kindly donated by Dr. Arthur Weiss (Department of Immunology, University of California, San Francisco, San Francisco, CA). pSVSH2-Fyn, containing mutant Fyn lacking amino acids 144–248, was kindly provided by Drs. Nicolas Dunant and Kurt Balmer-Hofer (Friedrich Miescher Institute, Basel, Switzerland). pEGFP-N1 and rabbit polyclonal antibody against green fluorescent protein (GFP) were obtained from Clontech. Anti–CD8 monoclonal antibody solution and high purity digitonin were from Calbiochem. Protein A–agarose and protein A/G⁺ agarose beads and antiphosphotyrosine (PY99) monoclonal antibody solution were purchased from Santa Cruz Biotechnology. DL--Hydroxymyristic acid (2-hydroxytetradecanoic acid), defatted BSA, and filipin were from Sigma Chemical Co. and n-octylglucoside was from Boehringer Mannheim. Tran³⁵S-label and ¹²⁵I-NaI were from DuPont-NEN. Synthesis and radioiodination of IC16 (16-iodohexadecanoic acid) and IC13 (13-iodotridecanoic acid) fatty acid analogues were performed as previously described (2).

Plasmid Construction
Construction of plasmids containing wild-type Fyn, G₂A-Fyn, C_3,6S-Fyn, and G_o-Fyn was described before (1, 41). For generation of K₇A-, K₉A-, K_7,9A-Fyn, and Lck(10)Fyn constructs, sense oligonucleotides were synthesized to encode the upstream region of pGEM3Z, an NcoI site, and either the first 11–14 amino acids of human Fyn, containing lysines to alanine substitutions at positions 7 and/or 9, or the first 10 amino acids of human Lck, followed by amino acids 11–16 of human Fyn. An antisense oligonucleotide was used corresponding to a region of the SH3 domain of Fyn (1). Sense and antisense primers were used with pGEM3Z-Fyn as a template to generate mutant cDNAs, which were digested with NcoI and BstXI to produce 76-bp fragments that were used to replace the corresponding fragments of Fyn in pSP65. A G₂A-FynKRas construct was generated by PCR using a sense oligonucleotide encoding nucleotides 1110–1130 of human Fyn containing a unique BglII site, and an antisense oligonucleotide corresponding to the last 18 nucleotides of Fyn, followed by the last 54 nucleotides of KRas4B, a stop codon, and a SalI site. The primers were used with pGEM3Z-Fyn as a template. The PCR product was digested with BglII and SalI to produce a 500-bp fragment that was used to replace a corresponding carboxy-terminal fragment of G₂A-Fyn in pSP65. All Fyn constructs in pSP65 were subsequently digested with EcoRI and SalI, and ligated into pCMV5. FynKRas was subsequently generated by digestion of pCMV5-G₂A-FynKRas with BglII and SalI, followed by ligation into BglII and SalI cut pCMV5-Fyn. G₂A,C₃S-FynKRas was generated by PCR, with pGEM3Z-Fyn as a template, using a sense oligonucleotide encoding an NcoI site followed by the first eight amino acids of human Fyn, containing a glycine-to-alanine substitution at position 2 and a cysteine-to-serine substitution at position 3, and an antisense oligonucleotide corresponding to the SH3 domain of Fyn (1). The PCR product was digested with NcoI and BstXI to generate a 76-bp fragment that was used to replace the corresponding fragment of pSP65-FynKRas. G₂A,C₃S-FynKRas subcloned into pCMV5 as described above. SH2-Fyn was subcloned into pSP65 by digestion of pSVSH2-Fyn with BstXI and BstE2 and ligation into BstXI- and BstE2-digested pSP65, and subcloned into pCMV5, as described above. K₂₉₉M-Fyn and R₁₇₆K-Fyn constructs were generated using the Quickchange site-directed mutagenesis kit (Stratagene Inc.). Fyn(16)-GFP was generated by PCR, using a sense oligonucleotide, encoding an EcoRI site followed by the first 16 amino acids of human Fyn fused in frame to amino acid 2 of eGFP, and an antisense oligonucleotide corresponding to the carboxy terminus of eGFP and an XbaI site. These primers were used with pEGFP-N1 as a template to generate a 1.6-kb DNA fragment that was digested with EcoRI and XbaI, followed by ligation into pCMV5.

Cell Culture and Transfection
COS-1 cells (American Type Culture Collection) were cultured and transfected as previously described (41). For cotransfection experiments with Fyn and NMT, 2 µg Fyn cDNA was used with 4 or 10 µg NMT cDNA (ratios 1:2 and 1:5). For CD8- coimmunoprecipitation experiments, 5 µg pEFBOS-CD8- was used with 5 µg pCMV5-Fyn construct and 10 µg pCMV5-NMT or pCMV5.

Metabolic Radiolabeling, Cell Fractionation and Pretreatment with 2-Hydroxymyristate and Filipin
Transfected COS-1 cells were starved for 1 h at 37°C in DMEM minus methionine/cysteine, supplemented with 2% dialyzed FBS, and labeled for 4 h at 37°C with 25 µCi/ml Tran³⁵S-label. For radiolabeling with fatty acid analogues, cells were starved for 1 h at 37°C in DMEM containing 2% dialyzed FBS, followed by radiolabeling for 4 h at 37°C with either 25 µCi/ml ¹²⁵I-IC13 or ¹²⁵I-IC16 (1, 41). Fractionation into cytosolic (S100) and total membrane (P100) fractions and extraction with the nonionic detergent Triton X-100 was performed as described previously (41). 2-Hydroxymyristate was stored as a 100-mM stock solution in DMSO and used for experiments at 1 mM in DMEM containing 1% defatted BSA. Before addition to cells, 1 mM 2-hydroxymyristate solution was sonicated briefly and filtered to remove any undissolved myristate analogue. After preincubation for 2 h at 37°C, DMEM containing 5% FBS was added, followed by overnight incubation at 500 µM 2-hydroxymyristate. Where indicated, cells were pretreated for 1 h at 37°C with 10 µg/ml filipin in DMEM containing 1% defatted BSA.

Immunoprecipitation, Gel Electrophoresis, and Quantitation of Fatty Acylation
For immunoprecipitation, each clarified lysate in RIPA buffer (10 mM Tris/HCl, pH 8.0, 150 mM NaCl, 1 mM EDTA, 1% Triton X-100, 0.1% SDS, 1% deoxycholate) was mixed with 3 µl anti–Fyn or 3 µl anti–GFP and 10 µl protein A–agarose solution, and incubated for 2–12 h at 4°C. Immunoprecipitates were washed twice with RIPA buffer, once with STE (50 mM Tris/HCl, pH 7.4, 150 mM NaCl, 1 mM EDTA), resuspended in SDS sample buffer containing 0.1 M DTT, and applied to SDS-PAGE. Radiolabeled proteins in dried gels were visualized by exposure for 8–24 h to X-Omat or BioMax film (Eastman Kodak Co.) or to PhosphorImager screens. Quantitation of radiolabeled proteins was performed using the ImageQuant software provided with the PhosphorImager system (Molecular Dynamics, Inc.). In each labeling experiment, constructs were labeled in duplicate with ¹²⁵I-IC13, ¹²⁵I-IC16, or Tran³⁵S-label, and the mean of the duplicates was calculated and used as the value for each individual experiment. Numbers were corrected for the background in each individual lane of the gel. Efficiency of myristoylation was calculated as ¹²⁵I-IC13 incorporation per unit of ³⁵S-label, which is accurate since all Fyn constructs used in this report (see Table I) contain identical amounts of methionines and cysteines. Numbers for myristoylation of mutant constructs were expressed relative to wild-type Fyn within each experiment. Each construct was analyzed in two to four experiments.

CD8- Coimmunoprecipitation Experiments

	Results

Top Abstract Materials and Methods Results Discussion References

 
Replacement of Lysines 7 and 9 in Fyn Results in Reduced Fatty Acylation and Membrane Anchoring
The first set of experiments was designed to quantitatively assess the contributions of lysine residues within the Fyn SH4 motif towards fatty acylation. COS-1 cells were transfected with cDNAs encoding either wild-type Fyn, G₂A-Fyn, or the K_7,9A-Fyn construct, in which lysines at positions 7 and 9 are replaced by alanine residues (Table I). Radiolabeling with Tran³⁵S-label, followed by immunoprecipitation of Fyn, SDS-PAGE and autoradiography, showed that all constructs were expressed at similar levels (Fig. 1). The K_7,9A-Fyn construct displayed moderately elevated levels of expression and migrated as a doublet (Fig. 1). Wild-type Fyn was labeled with both ¹²⁵I-IC13 (a myristate analogue) and ¹²⁵I-IC16 (a palmitate analogue), while G₂A-Fyn was not (Fig. 1, and Table II), as described previously (1, 41, 43). Although the K_7,9A-Fyn construct contains both the glycine at position 2 and the cysteine at position 3 required for efficient myristoylation and palmitoylation of Fyn (1, 41, 43), levels of ¹²⁵I-IC13 and ¹²⁵I-IC16 incorporation were drastically reduced (Fig. 1). In subsequent experiments, K₇A-Fyn and K₉A-Fyn mutants, containing alanine replacements of either lysine 7 or 9, were included to analyze the relevance of the individual lysines for fatty acylation. Radiolabeling with Tran³⁵S-label and ¹²⁵I-IC13, followed by calculation of expression levels and relative myristoylation (Table II), showed that mutation of lysine 7 or 9 individually reduced myristoylation of Fyn by 51 and 40%, respectively (Table II). Myristoylation of the double mutant, K_7,9A-Fyn, was inhibited by 83% (Table II), implying that the effect of each lysine mutation on myristoylation is additive. In agreement with the dependence of palmitoylation on myristoylation, the level of ¹²⁵I-IC16-palmitate labeling of K_7,9A-Fyn was also found to be reduced to 22 ± 3% (n = 4) of wild-type levels.

View larger version (16K): [in this window] [in a new window] [Download PPT slide]   Figure 1 Fatty acylation of Fyn, G2A-Fyn, and K7,9A-Fyn in COS-1 cells. COS-1 cells were transfected with cDNAs encoding wild-type Fyn, G2A-Fyn, and K7,9A-Fyn, and radiolabeled with either Tran35S-label, 125I-IC13, or 125I-IC16. Cell lysates were immunoprecipitated with anti–Fyn antibody and analyzed by SDS-PAGE and autoradiography. Gels were exposed to film for 8–24 h, and strips corresponding to the region of the gel containing p59Fyn are shown. No other radiolabeled proteins were apparent on the gel.

Since fatty acylation of Fyn is essential for membrane binding (1, 41, 43), the reduced levels of fatty acid modification of K_7,9A-Fyn would be expected to alter the subcellular distribution of this construct. Transfected cells expressing the various Fyn constructs were radiolabeled with Tran³⁵S-label, ¹²⁵I-IC13 or ¹²⁵I-IC16, followed by homogenization and fractionation into high-speed supernatant (S100) and membrane (P100) fractions, and the distribution of Fyn was analyzed. Fig. 2 shows that more than 95% of wild-type Fyn was recovered from the membrane fraction as dually acylated protein, whereas 75% of G₂A-Fyn was recovered from the soluble fraction, in agreement with previous results (1, 41, 43). In addition, slightly more than 50% of K_7,9A-Fyn was found in the soluble fraction (Fig. 2 B), specifically consisting of the protein band with the slower migration, that is neither myristoylated nor palmitoylated (A). The reason for this difference in migration is not clear, and it cannot be explained simply by the absence of fatty acylation since the G₂A-Fyn mutant does not show this effect. The remainder of K_7,9A-Fyn was recovered from the membrane fraction as dually acylated protein (Fig. 2 A). The calculated ratio of ¹²⁵I-IC13 label to Tran³⁵S-labeled in the P100 fraction was 25% lower for K_7,9A-Fyn compared with wild-type Fyn (data not shown), implying that some of the protein in the membrane fraction is not acylated. This is confirmed by the results with G₂A-Fyn, for which 25% of the protein is found in the membrane pellet, even though none of the protein is fatty acylated (Fig. 2 and Table II).

View larger version (16K): [in this window] [in a new window] [Download PPT slide]   Figure 2 Fatty acylation and subcellular distribution of Fyn, G2A-Fyn, and K7,9A-Fyn in COS-1 cells. (A) Transfected cells were radiolabeled with either Tran35S-label, 125I-IC13, or 125I-IC16. Cells were homogenized and fractionated into S100 (S) and P100 (P) fractions, followed by immunoprecipitation, SDS-PAGE, and autoradiography. Gels were exposed to film for 8–24 h. (B) Quantitation of the subcellular distribution of 35S-labeled wild-type and mutant Fyn by PhosphorImaging. Gels were exposed to PhosphorImager screens for 8–24 h. Values represent the mean of four independent experiments.

View larger version (25K): [in this window] [in a new window] [Download PPT slide]   Figure 3 Myristoylation of wild-type Fyn and K7,9A-Fyn coexpressed in COS-1 cells with wild-type or mutant NMT. Cotransfection of Fyn and NMT constructs in COS-1 cells was performed using 2 µg Fyn cDNA and 4 µg NMT cDNA. Radiolabeling of transfected cells, followed by immunoprecipitation, SDS-PAGE, and autoradiography was performed as described in Materials and Methods.

View larger version (15K): [in this window] [in a new window] [Download PPT slide]   Figure 4 Myristoylation efficiency and subcellular distribution of wild-type Fyn and K7,9A-Fyn after cotransfection in COS-1 cells with varying amounts of NMT cDNA. Cotransfection of Fyn and NMT constructs in COS-1 cells was performed as described in Materials and Methods, using 2 µg Fyn cDNA and 0, 4, or 10 µg NMT cDNA. Radiolabeling of cells transfected with (A) wild-type Fyn or (B) K7,9A-Fyn, followed by immunoprecipitation, SDS-PAGE, and quantitation of 125I-IC13 incorporation per unit 35S-labeled protein by PhosphorImaging was performed as described in Table II. Values are expressed relative to wild-type Fyn, expressed in the absence of exogenous NMT, and numbers represent the mean of four independent experiments. (C) Radiolabeling of cells transfected with 2 µg Fyn or K7,9A-Fyn cDNA and 4 µg NMT cDNA, followed by homogenization and subcellular fractionation. Analysis of protein distribution was performed as described in Fig. 2. Values represent the mean of four independent experiments.

Coimmunoprecipitation of Fyn with the Chain of the TCR Depends on the Fatty Acylation Status of Fyn
The ability to manipulate fatty acylation of Fyn provided us with a unique opportunity to quantitate the individual contributions of the fatty acids and the surrounding amino acids towards interactions of Fyn with other membrane bound proteins. We chose to evaluate the interactions of Fyn with the chain of the TCR complex as a model system. COS-1 cells were cotransfected with cDNAs for Fyn and CD8-, a chimeric construct containing the extracellular and transmembrane regions of CD8, fused to the cytoplasmic tail of the TCR chain (16). Cells were lysed in a 1% digitonin lysis buffer (10, 33) and subjected to immunoprecipitation with anti–CD8 monoclonal antibody. Incubation with protein A/G⁺ agarose beads alone was used as a negative control. When anti–CD8 immunoprecipitates were analyzed by Western blotting using polyclonal anti– Fyn antibody, a signal for Fyn was obtained using lysates from cells coexpressing Fyn and CD8- (Fig. 5 A, lane 3). Relative to the amount of wild-type Fyn, only marginal amounts (<5%) of G₂A-Fyn and C_3,6S-Fyn were detected after immunoprecipitation with anti–CD8 antiserum (Fig. 5, A, lanes 5 and 7, and B). Since G₂A-Fyn is neither myristoylated nor palmitoylated and C_3,6S-Fyn is myristoylated but not palmitoylated (1, 43), these data indicate that fatty acylation of Fyn with both myristate and palmitate is required for association of Fyn with CD8-. K_7,9A-Fyn was also impaired (70%) in its ability to coimmunoprecipitate with CD8- (Fig. 5), a result similar to that obtained by Gauen et al. (11) for association of K_7,9A-Fyn with a VSV G- chimera. However, the level of coimmunoprecipitation of K_7,9A-Fyn with CD8- could be increased twofold by overexpression of exogenous NMT (Fig. 5, A, lane 11, and B) and this correlates well with the twofold increase in myristoylation levels (Fig. 4 B). This gain of function experiment indicates that the presence of lysine residues at positions 7 and 9 in Fyn is not required per se for an interaction with the chain, but rather for efficient fatty acylation of Fyn. In addition, G_o-Fyn (41) and Lck(10)Fyn, fusion proteins in which the first 10 amino acids of Fyn are replaced with those of human G_o or human Lck (Table I) were analyzed. Both constructs are efficiently dually fatty acylated (see reference 41 and Table II), yet their NH₂-terminal sequences are distinct from that of Fyn outside the met-gly-cys motif (Table I). As depicted in Fig. 5 B, the levels of G_o-Fyn and Lck(10)Fyn coimmunoprecipitating with CD8- were similar (90%) to that of wild-type Fyn (Fig. 5 B), providing two additional examples of the need for dual fatty acylation rather than specific lysine residues for interaction of Fyn with CD8-. Controls indicated that expression levels of CD8- and Fyn constructs were constant throughout the experiments (see Fig. 5 A).

View larger version (19K): [in this window] [in a new window] [Download PPT slide]   Figure 5 Coimmunoprecipita-tion of wild-type or mutant Fyn constructs with CD8-. (A) COS-1 cells were cotransfected with cDNAs encoding wild-type or mutant Fyn (see Table I), CD8-, and NMT where indicated. Cells were lysed in digitonin buffer and subjected to immunoprecipitation with anti– CD8 monoclonal antibody (+) or with protein A/G+ agarose beads alone (–). Immunoprecipitates were analyzed by SDS-PAGE and Western blotting using polyclonal anti–Fyn antibody (top). Subsequently, the blot was stripped and reprobed using anti–CD8 monoclonal antibody; the distribution of the 41-kD form of CD8- is shown (middle). After immunoprecipitation with anti–CD8 antibody, lysates were subjected to a second immunoprecipitation step, using polyclonal anti–Fyn antibody, followed by SDS-PAGE and Western blotting using monoclonal anti–Fyn antibody (bottom). (B) Levels of Fyn protein coimmunoprecipitating with CD8- were quantified by scanning of films. Films were exposed for different times to the blot and measurements were made in the linear range of the film. The measured values for coimmunoprecipitation with CD8- were corrected for total expression levels and values are expressed relative to the amount of wild-type Fyn that coimmunoprecipitates with CD8-. Given values represent the mean of two experiments.

Inhibition of Myristoylation, Membrane Binding, and CD8- Association of Wild-Type Fyn by Treatment with 2-Hydroxymyristate

View larger version (19K): [in this window] [in a new window] [Download PPT slide]   Figure 6 Myristoylation, subcellular distribution, and coimmunoprecipitation of Fyn with CD8- after 2-hydroxymyristate treatment. Transfected cells expressing Fyn were preincubated overnight with 500 µM 2-hydroxymyristate, as described in Materials and Methods. (A) Cells were radiolabeled in the absence (–) or presence (+) of 500 µM 2-hydroxymyristate with Tran35S-label, or 125I-IC13, and analyzed directly (left) or subjected to homogenization and subcellular fractionation, followed immunoprecipitation (right). (B) COS-1 cells were cotransfected with cDNAs for Fyn and CD8-, and incubated in the absence (–) or the presence (+) of 2-hydroxymyristate. Cells were lysed in digitonin buffer and coimmunoprecipitation of Fyn with CD8- was analyzed using anti–CD8 antibody (+) or protein A/G+ agarose beads alone (–).

Association of Fyn with Chain: The NH₂ Terminus of Fyn Alone Is Not Sufficient and Functional SH2- and SH1-kinase Domains Are Essential

View larger version (27K): [in this window] [in a new window] [Download PPT slide]   Figure 7 Analysis of the molecular determinants in Fyn required for coimmunoprecipitation with CD8-. (A) COS-1 cells were transfected with empty pCMV5 vector (lanes 1 and 2), cDNA encoding CD8- alone (lanes 3 and 4), Fyn alone (lanes 5 and 6), or cotransfected with both CD8- and Fyn (lanes 7, 8, 11, and 12). Cells were lysed in digitonin buffer and subjected to immunoprecipitation with (+) or without (–) monoclonal antibody against CD8 (lanes 1–10) or Fyn (lanes 11 and 12). In addition, immunoprecipitation was performed using a mixed digitonin lysate, derived from cells transfected separately with CD8- or Fyn (lanes 9 and 10). Immunoprecipitates were analyzed by SDS-PAGE and Western blotting using polyclonal anti–Fyn antibody. (B) COS-1 cells were transfected with Fyn(16)GFP cDNA and either lysed in RIPA buffer and subjected to immunoprecipitation using anti–GFP antibody (Total) or fractionated into 1% Triton X-100 soluble (S) or resistant (R) fractions before immunoprecipitation (left). For coimmunoprecipitation analysis, COS-1 cells were transfected with Fyn(16)GFP and CD8- cDNA, lysed in digitonin buffer, and subjected to immunoprecipitation with (+) or without (–) anti–GFP or anti–CD8 antibody (right). Immunoprecipitates were analyzed by SDS-PAGE and Western blotting using polyclonal anti–GFP. (C) COS-1 cells were transfected with cDNAs encoding CD8- and either wild-type Fyn, K299M-Fyn, SH2-Fyn, or R176K-Fyn. Digitonin lysates were subjected to immunoprecipitation with anti–CD8 antibody (left) or anti–Fyn monoclonal antibody (right) and immunoprecipitates were analyzed by SDS-PAGE and Western blotting with anti–Fyn antibody. The locations of full length Fyn and SH2-Fyn are indicated by the arrows. The weak signal in the K299M-Fyn lane (left) may be accounted for by phosphorylation of CD8- by endogenous Fyn (see Fig. 8 A, legend).

View this table: [in this window] [in a new window]   Table III Quantitative Analysis of Coimmunoprecipitation of Fyn with CD8-

Association of Fyn with Chain Requires Phosphorylation of ITAMs by Fyn

View larger version (18K): [in this window] [in a new window] [Download PPT slide]   Figure 8 Analysis of the molecular interactions between Fyn and CD8-. (A) COS-1 cells were transfected with cDNAs encoding CD8- and either pCMV5, wild-type Fyn, K299M-Fyn, SH2-Fyn, or R176K-Fyn. Transfected cells were lysed in RIPA buffer and were subjected to immunoprecipitation with anti– CD8 antibody, followed by Western blotting analysis using antiphosphotyrosine (-PTyr) monoclonal antibody (top). As controls for expression levels, transfected cells were radiolabeled with Tran35S-label (bottom), lysed in RIPA buffer, and subjected to immunoprecipitation with anti–CD8 antibody, followed by SDS-PAGE and autoradiography. CD8- expressed in COS-1 cells is present in three forms that migrate at 36, 38, and 41 kD, respectively, as indicated by the arrows. The 41-kD form represents the main tyrosine phosphorylated band. Overexposure of the blot in the top row revealed a low level of phosphorylation of CD8- in the pCMV5 and K299M lanes, presumably reflecting the activity of endogenous Fyn or other kinases. (B) COS-1 cells were transfected with cDNAs encoding wild-type Fyn and either CD8-, CD8-T76, or CD8-4F. Antiphosphotyrosine Western blotting and radiolabeling were performed as described in A. Truncated CD8-T76 was present in one main form that migrated at 40 kD while the main radiolabeled form of CD8-4F migrated at 35 kD, as indicated by the arrows. (C) COS-1 cells were transfected as described in B and coimmunoprecipitation analysis of Fyn with CD8- constructs was performed as described in Fig. 7 C, legend.

Association of Fyn with CD8- Is Stabilized in Membrane Rafts

View larger version (18K): [in this window] [in a new window] [Download PPT slide]   Figure 9 Membrane binding, Triton X-100 sensitivity, and coimmunoprecipitation of fatty acylated and farnesylated Fyn constructs. (A) COS-1 cells were transfected with cDNAs encoding wild-type Fyn, FynKRas, or G2A,C3S-FynKRas. Transfected cells were radiolabeled with Tran35S-label, homogenized, and fractionated as described in Materials and Methods. Distribution into the P100 fraction was quantitated by phosphorimaging. Values represent the mean of two experiments. (B) COS-1 cells were transfected as described in A, followed by fractionation into 1% Triton X-100 soluble (S) or resistant (R) fractions. Distribution of Fyn constructs into the TX100 resistant fraction was quantitated after immunoprecipitation by Western blotting analysis, as described in Materials and Methods. Values represent the mean of two experiments. (C) COS-1 cells were transfected as described in A and coimmunoprecipitation analysis of Fyn protein with CD8- was performed as described in Fig. 7 C, legend.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Our results show that, as previously established for v-Src (6, 19), lysine 7 is required for efficient myristoylation of Fyn (Table II). In addition, we show that lysine 9 plays an important role in guiding effective myristoylation of Fyn (Table II). Interestingly, the effects of the individual lysine replacements add up to the total effect observed with the double K_7,9A-Fyn mutant (Fig. 1, and Table II), suggesting that each lysine residue plays an independent role. The conclusion that these lysines are directly involved in a myristoylation event is further substantiated by our finding that the K_7,9A-Fyn myristoylation defect is specifically reversed by coexpression with wild-type human NMT, but not with enzymatically impaired H₂₁₈N-NMT (28) (Figs. 3 and 4).

Reversal of the K_7,9A-Fyn myristoylation defect by additional exogenous NMT in our experiments was almost complete (Fig. 4 B). In the experiments described here, we have used cDNA encoding a 49-kD form of human NMT (28), which has full enzymatic activity in vitro and is capable of functionally complementing myristoylation deficiency in yeast (9). Additional cellular forms of NMT, with higher molecular weights (60 kD) and different intracellular distribution patterns, have been observed (14), and recently a second mammalian NMT was characterized (13). Most notably, missing from the 49-kD form of NMT (9, 28) is an NH₂-terminal sequence containing a polybasic motif that is proposed to function in ribosomal targeting of NMT (14), as well as other cotranslationally active enzymes, such as N-methionylaminopeptidases (21). We have observed that neither the 60-kD form nor the NMT 1 or 2 isoforms (13) reverse the myristoylation defect in K_7,9A-Fyn more efficiently than the 49-kD form (data not shown).

Lck is the only Src family member that lacks lysines at positions 7 and 9 (36, 37) and one might question whether myristoylation of Lck is impaired relative to the other Src-related kinases. Since quantitation of fatty acylation of full length Lck proved technically difficult, we used an Lck(10)Fyn fusion construct (Table I). Our results show that the fatty acylation profile of the Lck amino terminus is very similar to that of Fyn (Table II), despite the absence of lysines 7 and 9. We infer that in Lck the serine at position 6 (Table I), a preferred residue at this site for recognition by mammalian NMT (17) is sufficient to direct efficient fatty acylation of this sequence. If myristoylation levels of full length Lck were substoichiometric, one would expect that either its membrane association would not be complete or that additional factors (e.g., CD4) would be required to guide membrane binding of Lck. However, nearly all of the Lck in cells appears to be membrane bound (18, 46). Moreover, two recent studies have shown that plasma membrane targeting of Lck can be achieved in the absence of CD4 and that the first 10 amino acids of Lck are sufficient for plasma membrane binding (4, 46). These experiments imply that myristoylation and palmitoylation of full length Lck occur efficiently.

The NH₂ Terminus of Fyn Directs Fatty Acylation and Membrane Localization, but Does Not Specify an ITAM Binding Motif
Several earlier reports have described coimmunoprecipitation of the thymic isoform of Fyn with the TCR/CD3 complex (10, 12, 33). The association was only observed under mild detergent conditions and the exact nature of the interaction remained unclear. Recently, the first 10 amino acids of Fyn were shown to be essential for specific binding of Fyn to the subunit, as well as other chains of the TCR complex in heterologous systems (10). On the basis of mutagenesis experiments, it was concluded that the amino acids glycine 2, cysteine 3, and lysines 7 and 9 define a motif for binding to ITAMs and for plasma membrane localization (11).

Our results described here (Figs. 1–4), as well as earlier work from our group and others (1, 35, 41, 43), indicate that these amino acids within the Fyn SH4 domain are essential for optimal fatty acylation and membrane binding of Fyn. Using the coimmunoprecipitation of various Fyn constructs with a CD8- fusion protein (16) as a model, we present three lines of evidence to demonstrate that the Fyn SH4 domain does not represent a specific ITAM binding motif.

First, we show that the reduced coimmunoprecipitation of the K_7,9A-Fyn mutant with CD8- (Fig. 5, and reference 11) is specifically reversed by overexpression of NMT (Fig. 5). The effect of NMT overexpression is to increase fatty acylation and membrane binding of K_7,9A-Fyn (Figs. 3 and 4). This gain of function experiment clearly establishes that coimmunoprecipitation of Fyn with CD8- does not require lysines 7 and 9 per se, but their presence is crucial for directing efficient fatty acylation. This conclusion is further substantiated by the observations made with the G_o-Fyn and Lck(10)Fyn constructs, which coimmunoprecipitate with CD8- as efficiently as wild-type Fyn (Fig. 5 B). The NH₂-terminal sequences of G_o-Fyn and Lck(10)Fyn do not contain lysines at position 7 and 9 (Table I), but they are efficiently fatty acylated (reference 41, and Table I). Second, the loss of function experiment with 2-hydroxymyristate (Fig. 6) shows that, even in the presence of all the amino acids proposed to constitute the ITAM binding motif (glycine 2, cysteine 3, and lysines 7 and 9), coimmunoprecipitation of wild-type Fyn with CD8- can be ablated. Thus, loss of association of wild-type Fyn to CD8- coincides with a reduction of fatty acylation and membrane binding (Fig. 6). Third, Fyn(16)GFP did not coimmunoprecipitate with CD8- (Fig. 7 B), showing that the first 16 amino acids of Fyn are not sufficient for interaction with the ITAMs on , in agreement with the results of cross-linking studies (34). This implies that other protein determinants in Fyn are involved in mediating the interactions with chain. Indeed, coimmunoprecipitation of Fyn was observed to require both a functional kinase as well as an SH2 domain (Fig. 7 C).

Colocalization of Fyn and Chain in Cell Surface Rafts
Coimmunoprecipitation of Fyn with TCR subunits occurs only under mild detergent conditions (10, 12, 33), which has been taken as evidence for low affinity protein–protein interactions. Our findings with Fyn, and a recently growing interest in membrane microdomains (5, 38), suggests the involvement of additional mechanisms for stabilization of the interactions between Src kinases and TCR subunits, which is supported by several recent independent reports (24, 44, 45). In biological membranes, especially plasma membranes, phase-separated "rafts" exist, representing lipid domains enriched in cholesterol and sphingolipids that provide scaffolds for clustering of transmembrane and peripherally associated proteins (5, 38). These rafts or microdomains can be recovered from cells using mild detergent conditions (5). There is growing evidence that key components of TCR-mediated signaling events are localized to rafts. For example, palmitoylation of the T cell transmembrane protein LAT is essential for localization in rafts and T cell tyrosine phosphorylation events (45). Src family kinases, especially Fyn and Lck, are constitutively localized in rafts via dual fatty acylation motifs (35, 41, 43). Activation of the TCR results in specific accumulation of chains in plasma membrane rafts (24). In COS cells, 20% of CD8- is in the detergent-insoluble fraction (data not shown), similar to the distribution of the chain in resting T cells (7), and this may explain in part why only a limited amount (<20%) of total Fyn coimmunoprecipitates with CD8- in COS cells. The functional significance of raft localization is evidenced by the finding that disruption of cell surface rafts interferes with early T cell signaling events (44). These observations establish a connection between local accumulation of signaling molecules in plasma membrane rafts and regulated T cell signaling events.

Based on the results reported here and by others (35, 39, 41, 43), the following model emerges. Myristoylation and palmitoylation within the NH₂-terminal SH4 domain directs Fyn into detergent-resistant plasma membrane rafts and positions the downstream SH2 and kinase domains in close proximity to the TCR chain. Phosphorylation of the ITAMs by Fyn (Fig. 8) allows subsequent interaction between the phosphorylated ITAMs and the Fyn SH2 domain (Figs. 7 and 8). Accumulation of Fyn and the chain in rafts increases the local concentration of both proteins and drives their association. The stability and the extent of Fyn SH2/ phosphotyrosine interaction is apparently dependent on the integrity of the rafts since treatment with octylglucoside and filipin, agents that disrupt rafts (5, 38), results in dissociation of the Fyn/ complex (Table III), presumably due to a decrease of the effective local protein concentrations. This implies that the Fyn SH2/ phosphotyrosine interaction is relatively weak, as found for several other SH2/phosphotyrosine interactions (20). In T cells, dissociation of the Fyn SH2 domain from the chain would make ITAM phosphotyrosine residues on accessible for binding to the SH2 domains of other signaling molecules, such as ZAP-70. This model explains why undermyristoylated and underpalmitoylated forms of Fyn, that are not efficiently membrane bound, as well as a farnesylated Fyn construct that is not enriched in membrane subdomains (Fig. 9), do not interact well with the chain. These studies illustrate that the role of the NH₂-terminal SH4 motif is to properly position Src kinases within specific locations of cellular membranes for optimal interaction of downstream Src homology domains with other membrane-bound signaling molecules.

	Acknowledgments

 
We thank Dr. Art Weiss for his generous gifts of CD8- plasmids. We are grateful to Raya Louft-Nisenbaum for technical assistance and Lori Klausner for secretarial support.

This work was supported by grant GM 57966 from the National Institutes of Health and grant BE235 from the American Cancer Society to M.D. Resh. M.D. Resh is an Established Scientist of the American Heart Association. W. van't Hof is a Miriam and Benedict Wolf Cancer Research fellow.

Submitted: 29 October 1998

Revised: 24 February 1999

Dr. van't Hof's present address is Pulmonary Research Laboratories, Division of Pulmonary and Critical Care Medicine, Weill Medical College of Cornell University, 1300 York Ave., F-401, New York, NY 10021.

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