In vitro synthesis of pp60v-src: myristylation in a cell-free system.

Deichaite, Ida; Casson, Lawrence P.; Ling, Huai-Ping; Resh, Marilyn D.

doi:10.1128/mcb.8.10.4295

Cited by 112 publications

(127 citation statements)

References 45 publications

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“…The detection of a broader reactive band corresponding to Calymmin, in both in vitro transcription-translation and embryo protein extracts, may suggest the existence of posttranslational modifications of the peptide both in vivo and in cell-free systems. This would agree with the various N-and mucin type Oglycosylation conserved motifs, and the high number of potential N-myristoylation sites found in the amino acid sequence of Calymmin (e.g., Deichaite et al, 1988).…”

Section: Protein Characterization and Cellular Localization Of Calymmsupporting

confidence: 77%

Molecular characterization of Calymmin, a novel notochord sheath‐associated extracellular matrix protein in the zebrafish embryo

Cerdà

Gründ

Franke

et al. 2002

Developmental Dynamics

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During the screening of a zebrafish postsomitogenesis embryo cDNA library, we have identified a cDNA corresponding to a novel type of protein localized to the notochordal sheath-associated extracellular matrix (ECM) of the embryo. The 4.049-kb mRNA encodes a predicted polypeptide of 1,207 amino acids (122 kDa, pI 10.50) with a potential signal peptide of 20 amino acids. After the signal peptide, the mature protein consists of 1,187 amino acids (119 kDa, pI 10.46), for which the name "Calymmin" (from Greek ␣ ␣, to envelop, to cover) is proposed. The Calymmin mRNA is highly and transiently expressed by the notochord cells of the embryo from the 10-to 12-somite stage to the pharyngula period (13 and 24 hours postfertilization, respectively), and light and electron microscopical immunolocalization analysis revealed that the protein was specifically localized within a granular and filamentous layer of the ECM compartment surrounding the notochord. In zebrafish no tail mutants (ntl tc41 ), in which the notochord precursor cells are present but fail to differentiate, the Calymmin protein was not detected, confirming the notochord origin of Calymmin. These results indicate that Calymmin is a novel constitutive protein of the ECM compartment associated to the perinotochordal sheath in the zebrafish embryo, which is specifically expressed by the differentiating notochord cells.

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Section: Protein Characterization and Cellular Localization Of Calymmsupporting

confidence: 77%

Molecular characterization of Calymmin, a novel notochord sheath‐associated extracellular matrix protein in the zebrafish embryo

Cerdà

Gründ

Franke

et al. 2002

Developmental Dynamics

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“…Since both NMTs and methionine aminopeptidases function cotranslationally while the nascent polypeptide chain is still attached to the ribosomes (20,36,37), it might be possible to speculate that these two enzymes may share similar restrictions with respect to their substrate specificities.…”

Section: Discussionmentioning

confidence: 99%

“…Since the in vitro translation system using rabbit reticulocyte lysate contains the components involved in cotranslational protein N-myristoylation and N-acetylation (17,19,20), the use of this system to study cotranslational protein modification seems to be appropriate. In fact, we previously demonstrated that tumor necrosis factor (TNF), a nonmyristoylated model protein, could be efficiently myristoylated in the in vitro trans-lation system when an N-myristoylation motif of Rasheed leukemia virus-Gag protein or G i1 ␣ protein was linked to the mature domain of TNF (21,22).…”

Section: From the Department Of Biological Chemistry And §Department mentioning

confidence: 99%

Amino Acid Residue Penultimate to the Amino-terminal Gly Residue Strongly Affects Two Cotranslational Protein Modifications, N-Myristoylation andN-Acetylation

Utsumi

Sato

Nakano

et al. 2001

Journal of Biological Chemistry

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To examine the amino-terminal sequence requirements for cotranslational protein N-myristoylation, a series of site-directed mutagenesis of N-terminal region were performed using tumor necrosis factor as a nonmyristoylated model protein. Subsequently, the susceptibility of these mutants to protein N-myristoylation was evaluated by metabolic labeling in an in vitro translation system or in transfected cells. It was found that the amino acid residue at position 3 in an N-myristoylation consensus motif, Met-Gly-X-X-X-Ser-X-X-X, strongly affected the susceptibility of the protein to two different cotranslational protein modifications, N-myristoylation and N-acetylation; 10 amino acids (Ala, Ser, Cys, Thr, Val, Asn, Leu, Ile, Gln, and His) with a radius of gyration smaller than 1.80 Å directed N-myristoylation, two negatively charged residues (Asp and Glu) directed N-acetylation, and two amino acids (Gly and Met) directed heterogeneous modification with both N-myristoylation and N-acetylation. The amino acid requirements at this position for the two modifications were dramatically changed when Ser at position 6 in the consensus motif was replaced with Ala. Thus, the amino acid residue penultimate to the N-terminal Gly residue strongly affected two cotranslational protein modifications, N-myristoylation and N-acetylation, and the amino acid requirements at this position for these two modifications were significantly affected by downstream residues.

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“…Because the mechanism for N-terminal myristoylation appears to be conserved in Drosophila (Deichaite et al, 1988;Ntwasa et al, 1997;Benting et al, 2000), it is likely that Nullo exists as a myristoylprotein in vivo.…”

Section: Nullo Is Modified By N-terminal Myristoylationmentioning

confidence: 99%

“…First, the consensus target for NMT activity appears to be well conserved between Drosophila and other organisms. Both Drosophila embryonic extracts and Schnieder cells have been shown to have an NMT activity that modifies myristoyl proteins from other organisms in a specific manner, and the corresponding NMT gene has been shown to be expressed before cellularization (Deichaite et al, 1988;Ntwasa et al, 1997;Benting et al, 2000). Second, the glycine to alanine mutation which blocks myristoylation in vitro has a striking effect on the subcellular localization of Nullo in vivo, suggesting that the N-myristoylation site is important for the targeting of Nullo to the plasma membrane.…”

Section: N-terminal Motifs Control the Localization Of Nullo Proteinmentioning

confidence: 99%

Conserved Domains of the Nullo Protein Required for Cell-Surface Localization and Formation of Adherens Junctions

Hunter

Sung

Schejter

et al. 2002

MBoC

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During cellularization, the Drosophila melanogasterembryo undergoes a transition from syncytial to cellular blastoderm with the de novo generation of a polarized epithelial sheet in the cortex of the embryo. This process couples cytokinesis with the establishment of apical, basal, and lateral membrane domains that are separated by two spatially distinct adherens-type junctions. Innullo mutant embryos, basal junctions fail to form at the onset of cellularization, leading to the failure of cleavage furrow invagination and the generation of multinucleate cells. Nullo is a novel protein that appears to stabilize the initial accumulation of cadherins and catenins as they form a mature basal junction. In this article we characterize a nullo homologue from D. virilis and identify conserved domains of Nullo that are required for basal junction formation. We also demonstrate that Nullo is a myristoylprotein and that the myristate group acts in conjunction with a cluster of basic amino acids to target Nullo to the plasma membrane. The membrane association of Nullo is required in vivo for its role in basal junction formation and for its ability to block apical junction formation when ectopically expressed during late cellularization.

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In vitro synthesis of pp60v-src: myristylation in a cell-free system.

Cited by 112 publications

References 45 publications

Molecular characterization of Calymmin, a novel notochord sheath‐associated extracellular matrix protein in the zebrafish embryo

Molecular characterization of Calymmin, a novel notochord sheath‐associated extracellular matrix protein in the zebrafish embryo

Amino Acid Residue Penultimate to the Amino-terminal Gly Residue Strongly Affects Two Cotranslational Protein Modifications, N-Myristoylation andN-Acetylation

Conserved Domains of the Nullo Protein Required for Cell-Surface Localization and Formation of Adherens Junctions

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