2001
DOI: 10.1074/jbc.m102555200
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A Non-Golgi α1,2-Fucosyltransferase That Modifies Skp1 in the Cytoplasm of Dictyostelium

Abstract: Skp1 is a subunit of the SCF-E3 ubiquitin ligase that targets cell cycle and other regulatory factors for degradation. In Dictyostelium, Skp1 is modified by a pentasaccharide containing the type 1 blood group H trisaccharide at its core. To address how the third sugar, fucose ␣1,2-linked to galactose, is attached, a proteomics strategy was applied to determine the primary structure of FT85, previously shown to copurify with the GDPFuc:Skp1 ␣1,2-fucosyltransferase. Tryptic-generated peptides of FT85 were sequen… Show more

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Cited by 34 publications
(59 citation statements)
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“…The null mutant of PpVps15 was provided by Dr. J. Cregg (Keck Graduate Institute; Stasyk et al, 1999). PpVAC8 was cloned from genomic DNA using degenerate primers combined with linker-mediated PCR (van Der Wel et al, 2001). The entire gene was sequenced and assembled (NCBI accession number AY886543).…”
Section: Isolation Of Gsa Mutants and Cloning Of Gsa Genes By Restricmentioning
confidence: 99%
See 1 more Smart Citation
“…The null mutant of PpVps15 was provided by Dr. J. Cregg (Keck Graduate Institute; Stasyk et al, 1999). PpVAC8 was cloned from genomic DNA using degenerate primers combined with linker-mediated PCR (van Der Wel et al, 2001). The entire gene was sequenced and assembled (NCBI accession number AY886543).…”
Section: Isolation Of Gsa Mutants and Cloning Of Gsa Genes By Restricmentioning
confidence: 99%
“…The site of insertion of the pREMI-Z and identification of the disrupted gene was done as described . Based on the genomic sequences around the pREMI-Z insertion site that was isolated along with the pREMI-Z vector from the R19 mutant, GSA14 was cloned and sequenced from genomic DNA using a linker-mediated PCR method previously described (van Der Wel et al, 2001). We were able to completely assemble the GSA14 gene (National Center for Biotechnology Information [NCBI] accession number AY075105) and show it encodes a protein homologous to ScAtg9 of S. cerevisiae, using the adapted ATG nomenclature for those genes uniquely essential for autophagy .…”
Section: Isolation Of Gsa Mutants and Cloning Of Gsa Genes By Restricmentioning
confidence: 99%
“…Notable in this regard is the use of 18 O incorporation at the carboxyl-termini of peptides during protein hydrolysis [14 -17]. For underivatized peptides, ESI has found use for de novo sequencing under a variety of conditions, which include collision-induced dissociation (CID) in the triple quadrupole mass analyzer [18 -20] and the QqTOF mass analyzer [18,19,[21][22][23][24][25][26], resonant excitation in the quadrupole ion trap mass analyzer [14,[27][28][29], and electron capture dissociation in the Fourier transform ion cyclotron resonance mass analyzer [30 -34]. MALDI de novo sequencing has been carried out using CID and metastable decay in single- [35] and double-stage [36 -39] TOF instruments and with CID in QqTOF instruments [40 -44].…”
mentioning
confidence: 99%
“…The previously reported peptide sequence VRGNPT CLRNHDGI (38) was found to be encoded perfectly by a 309-nucleotide (nt) sequence present in a database of random sequences of shotgun-cloned Dictyostelium genomic DNA (gDNA) available at the time. Primers derived from this nucleotide sequence were used to clone additional gDNA (unpublished data) using inverse PCR and linker-mediated PCR (20,27,28). Segments of the new sequences matched other gDNA sequences in the databases.…”
Section: Methodsmentioning
confidence: 99%