The Cytoplasmic Domain of Human FcγRIa Alters the Functional Properties of the FcγRI·γ-Chain Receptor Complex

Edberg, Jeffrey C.; Yee, Arthur M.F.; Rakshit, Diptendu S.; Chang, David J.; Gokhale, Jayashree A.; Indik, Zena K.; Schreiber, Alan D.; Kimberly, Robert P.

doi:10.1074/jbc.274.42.30328

Cited by 36 publications

(48 citation statements)

References 45 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Furthermore, 10 g/ml of mouse F(abЈ) 2 of IgG did not affect the standard curves. The data were confirmed by an additional method described by Edberg et al (20). Wells of tissue culture plates were coated with absorbed protein (10 g/ml of goat F(abЈ) 2 of anti-mouse F(abЈ) 2 of IgG) in carbonate-bicarbonate buffer (Sigma) for 30 min at 37°C and overnight at 4°C.…”

Section: Cytokine Elisamentioning

confidence: 90%

“…With regard to this observation, recent evidence suggests that the cytoplasmic domain of Fc␥RI␣ may recruit distinct signaling elements to the receptor complex (20). It has been shown by comparison of responses in wild-type human Fc␥RI␣ with a cytoplasmic domain deletion mutant of Fc␥RI␣ expressed at comparable levels in stable transfectants of the murine macrophage cell line that the Fc␥RI␣-␥-chain complex-induced responses, such as IL-6 production and phagocytosis, are altered (20). The basis for these differences is still unknown, but this might explain significant enhancement of some cytokine mRNAs expression via Fc␥RI aggregation compared with Fc⑀RI aggregation.…”

Section: Discussionmentioning

confidence: 99%

See 1 more Smart Citation

A Comparison of Mediators Released or Generated by IFN-γ-Treated Human Mast Cells Following Aggregation of FcγRI or FcεRI

Okayama

Hagaman

Metcalfe

2001

The Journal of Immunology

View full text Add to dashboard Cite

The high affinity receptor for IgG (FcγRI, CD64) is expressed on human mast cells, where it is up-regulated by IFN-γ and, thus, may allow mast cells to be recruited through IgG-dependent mechanisms in IFN-γ-rich tissue inflammation. However, the mediators produced by human mast cells after aggregation of FcγRI are incompletely described, and it is unknown whether these mediators are distinct from those produced after activation of human mast cells via FcεRI. Thus, we investigated the release of histamine and arachidonic acid metabolites and examined the chemokine and cytokine mRNA profiles of IFN-γ-treated cultured human mast cells after FcγRI or FcεRI aggregation. Aggregation of FcγRI resulted in histamine release and PGD2 and LTC4 generation. These responses were qualitatively indistinguishable from responses stimulated via FcεRI. Aggregation of FcεRI or FcγRI led to an induction or accumulation of 22 cytokine and chemokine mRNAs. Among them, seven cytokines (TNF-α, IL-1β, IL-5, IL-6, IL-13, IL-1R antagonist, and GM-CSF) were significantly up-regulated via aggregation of FcγRI compared with FcεRI. TNF-α mRNA data were confirmed by quantitative RT-PCR and ELISA. Furthermore, we confirmed histamine and TNF-α data using IFN-γ-treated purified human lung mast cells. Thus, aggregation of FcγRI on mast cells led to up-regulation and/or release of three important classes of mediators: biogenic amines, lipid mediators, and cytokines. Some cytokines, such as TNF-α, were released and generated to a greater degree after FcγRI aggregation, suggesting that selected biologic responses of mast cells may be preferentially generated through FcγRI in an IFN-γ-rich environment.

show abstract

Section: Cytokine Elisamentioning

confidence: 90%

Section: Discussionmentioning

confidence: 99%

A Comparison of Mediators Released or Generated by IFN-γ-Treated Human Mast Cells Following Aggregation of FcγRI or FcεRI

Okayama

Hagaman

Metcalfe

2001

The Journal of Immunology

View full text Add to dashboard Cite

show abstract

“…Cell Culture and Reagents-The murine macrophage cell line P388D1 (obtained from American Type Culture Collection, Manassas, VA) was stably transfected with a cDNA encoding human Fc␥RIa (WT) or a mutant form of Fc␥RIa containing a stop codon after the first amino acid of the cytoplasmic domain (Lys 315 3 Stop 315) (CYϪ) as we have described previously (8,22). Fc␥RIa constructs encoding serine to alanine mutations (S328A/S331A, S339A/S340A, and S328A/S331A/ S339A/S340A (S 4 3 A 4 )) were prepared by overlap PCR and stably transfected as described previously (22,24).…”

Section: Methodsmentioning

confidence: 99%

“…However, the ␣-chain is sufficient for endocytosis (7,9). Whereas expression of the Fc␥RIa ␣-chain without a CY domain can also induce pseudopod extension and endocytosis, recent data from our group and others have provided the first evidence that the ␣-chain of Fc␥RIa can alter receptor function downstream of IgG binding (21)(22)(23). Expression of an Fc␥RIa ␣-chain lacking the CY domain in a murine macrophage cell line results in quantitative differences in the phagocytic and endocytic capacity of the ␣␥ 2 receptor complexes compared with wild-type Fc␥RI.…”

mentioning

confidence: 98%

The CY Domain of the FcγRIa α-Chain (CD64) Alters γ-Chain Tyrosine-based Signaling and Phagocytosis

Edberg

Qin

Gibson

et al. 2002

Journal of Biological Chemistry

Self Cite

View full text Add to dashboard Cite

Although the cytoplasmic domain of the human Fc␥RIa ␣-chain lacks tyrosine-based phosphorylation motifs, it modulates receptor cycling and receptorspecific cytokine production. The cytoplasmic domain of Fc␥RIa is constitutively phosphorylated, and the inhibition of dephosphorylation with okadaic acid, an inhibitor of type 1 and type 2A protein serine/threonine phosphatase, inhibits both receptor-induced activation of the early tyrosine phosphorylation cascade and receptor-specific phagocytosis. To explore the basis for these effects of the cytoplasmic domain of Fc␥RIa, we developed a series of human Fc␥RIa molecular variants, expressed in the murine macrophage cell line P388D1, and demonstrate that serine phosphorylation of the cytoplasmic domain is an important regulatory mechanism. Truncation of the cytoplasmic domain and mutation of the cytoplasmic domain serine residues to alanine abolish the okadaic acid inhibition of phagocytic function. In contrast, the serine mutants did not recapitulate the selective effects of cytoplasmic domain truncation on cytokine production. These results demonstrate for the first time a direct functional role for serine phosphorylation in the ␣-chain of Fc␥RIa and suggest that the cytoplasmic domain of Fc␥RI regulates the different functional capacities of the Fc␥RIa-receptor complex.The ␥-chain, initially described as a component of the Fc⑀RI signaling complex, is able to form multichain complexes with the ligand-binding ␣-chain of several Fc receptors (1-3). The Fc␥RIa (CD64), Fc␥RIIIa (CD16A), Fc␣RI (CD89), and Fc⑀RI ␣-chains associate with the ␥-chain as a common molecule in signal transduction. The stoichiometry of the assembly of the receptor complex is generally ␣␥ 2 , except in mast cells, which may have Fc⑀RI and Fc␥RIIIa complexes where there is, in addition, a ␤ chain (␣␤␥ 2 ) (4 -6). In all of these Fc receptor complexes, the ␥-chain with its tyrosine activation motif (ITAM) is necessary for receptor signaling (7-9). In the case of Fc⑀RI, the ␤-chain serves as an amplifier of receptor function (10, 11).Fc␥RIa, a receptor with high affinity for IgG (10 9 M Ϫ1 ) (12), has received attention over the past few years as a potential therapeutic target in malignancy. Targeting of tumors to Fc␥RI with bispecific mAbs 1 can facilitate tumor killing via Fc␥RI-expressing macrophages, and therapeutic humanized bispecific reagents targeting human Fc␥RIa are currently in clinical trials (13-19). Bispecific mAb-based antigen targeting to Fc␥RI can also enhance antigen presentation by dendritic cells with clear applications to enhanced immunization strategies (20).Expression of the Fc␥RIa ␣-chain in the presence or absence of the ␥-chain has allowed an assessment of the functional capacity of each chain. For example, the ␥-chain is necessary for Fc␥RIa-mediated phagocytosis and Fc␥RIa-induced activation of tyrosine kinase activity (7-9). However, the ␣-chain is sufficient for endocytosis (7,9). Whereas expression of the Fc␥RIa ␣-chain without a CY domain can also induce pseudopod ext...

show abstract

“…The Fc␥RI cytosolic domain (Fc␥RI-CY) mediated MHC class II antigen presentation without active FcR ␥-chain signaling (10), whereas deletion of Fc␥RI-CY retarded kinetics of endocytosis and phagocytosis and abrogated Fc␥RI-triggered IL-6 secretion (11). Thus far, only actin-binding protein 280 (filamin A) has been described to bind Fc␥RI-CY under some conditions, but effects on receptor function have not been shown (12).…”

Section: A Ntibody (Ig) Complexes Can Induce Potent Immune Effector Fmentioning

confidence: 99%

Direct interaction between FcγRI (CD64) and periplakin controls receptor endocytosis and ligand binding capacity

Beekman

Bakema

Winkel

et al. 2004

Proc. Natl. Acad. Sci. U.S.A.

View full text Add to dashboard Cite

Fc␥RI depends for its biological function on both the intracellular domain of the ␣-chain and associated Fc receptor (FcR) ␥-chains. However, functional protein effectors of Fc␥RI's intracellular domain have not been identified. In this study, we identified periplakin (PPL) as a selective interacting protein for the intracellular tail of Fc␥RI but no other activatory FcRs. The interaction was confirmed by coimmunoprecipitation and blot-overlay assays. PPL and Fc␥RI colocalized at the plasma membrane in monocytes and cell transfectants, and both were up-regulated by IFN-␥. By expressing C-terminal PPL in transfectants, we established a pivotal role for this protein in Fc␥RI ligand binding, endocytosis, and antigen presentation. These data illustrate that intracellular protein interactions with a multisubunit FcR ␣-chain can confer unique properties to the receptor.

show abstract

The Cytoplasmic Domain of Human FcγRIa Alters the Functional Properties of the FcγRI·γ-Chain Receptor Complex

Cited by 36 publications

References 45 publications

A Comparison of Mediators Released or Generated by IFN-γ-Treated Human Mast Cells Following Aggregation of FcγRI or FcεRI

A Comparison of Mediators Released or Generated by IFN-γ-Treated Human Mast Cells Following Aggregation of FcγRI or FcεRI

The CY Domain of the FcγRIa α-Chain (CD64) Alters γ-Chain Tyrosine-based Signaling and Phagocytosis

Direct interaction between FcγRI (CD64) and periplakin controls receptor endocytosis and ligand binding capacity

Contact Info

Product

Resources

About