B-cell linker

Template:Short description Template:Cs1 config Template:Infobox gene B-cell linker (BLNK) protein is expressed in B cells and macrophages and plays a large role in B cell receptor signaling.^[1] Like all adaptor proteins, BLNK has no known intrinsic enzymatic activity.^[2] Its function is to temporally and spatially coordinate and regulate downstream signaling effectors in B cell receptor (BCR) signaling, which is important in B cell development.^[3] Binding of these downstream effectors is dependent on BLNK phosphorylation.^[4][5] BLNK is encoded by the BLNK gene^[4][6] and is also known as SLP-65,^[7] BASH,^[8] and BCA.^[9]

Structure and localization

BLNK consists of a N-terminal leucine zipper motif followed by an acidic region, a proline-rich region, and a C-terminal SH2 domain.^[10][1] The leucine zipper motif allows BLNK to localize to the plasma membrane, presumably by coiled-coil interactions with a membrane protein.^[1] This leucine zipper motif distinguishes BLNK from lymphoctye cytosolic protein 2, also known as LCP-2 or SLP-76, which plays a similar role in T cell receptor signaling.^[11] Although LCP-2 has an N-terminal heptad-like organization of leucine and isoleucine residues like BLNK, it has not been experimentally shown to have the leucine zipper motif.^[12] Recruitment of BLNK to the plasma membrane is also achieved by binding of the SH2 domain of BLNK to a non-ITAM phospho-tyrosine on the cytoplasmic domain of CD79A, which is a part of Igα and the B cell receptor complex.^[13][14][15]

Function

BLNK's function and importance in B cell development were first illustrated in BLNK deficient DT40 cells, a chicken B cell line.^[3] DT40 cells had interrupted B cell development: there was no calcium mobilization response in the B cell, impaired activation of the mitogen-activated protein (MAP) kinases p38, JNK, and somewhat inhibited ERK activation upon (BCR) activation as compared to wild type DT40 cells.^[3] In knockout mice, BLNK deficiency results in a partial block in B cell development,^[16][17] and in humans BLNK deficiency results in a much more profound block in B cell development.^[18][1]

Linker or adaptor proteins provide mechanisms by which receptors can amplify and regulate downstream effector proteins.^[2] BLNK is essential for normal B-cell development as part of the B cell receptor signaling pathway. [supplied by OMIM]^[6][19][20]

Evidence also suggests that BLNK may have tumor suppressive activity through its interaction with Bruton's tyrosine kinase (Btk) ^[21][22] and regulation of the pre-B cell checkpoint.^[10][23]

Phosphorylation and interactions

The acidic region of BLNK contains several inducibly phosphorylated tyrosine residues, at least five of which are found in humans.^[24] Evidence suggests that BLNK is phosphorylated by the tyrosine-protein kinase Syk after B cell receptor activation.^{[4][5][20][25]} Phosphorylation of these residues provides docking sites necessary for downstream protein-protein interactions between BLNK and the SH2 domain-containing proteins Grb2,^{[4][7][13][26]} PLCG2, Btk, the Vav protein family, and Nck.^[27][5][4] BLNK has also been shown to interact with SH3KBP1^[28] and MAP4K1.^[29] A more recent mass spectrometry study of BLNK in DT40 cells found that at least 41 unique serine, threonine, and tyrosine residues are phosphorylated on BLNK.^[30]

References

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Further reading

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External links

• Template:UCSC gene info