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Structural analyses of 4-phosphate adaptor protein 2 yield mechanistic insights into sphingolipid recognition by the glycolipid transfer protein family

  1. Author:
    Ochoa-Lizarralde, Borja
    Gao, Yong-Guang
    Popov, Alexander N
    Samygina, Valeria R [ORCID]
    Zhai, Xiuhong
    Mishra, Shrawan K
    Boldyrev, Ivan A
    Molotkovsky, Julian G
    Simanshu, Dhirendra [ORCID]
    Patel, Dinshaw J
    Brown, Rhoderick E
    Malinina, Lucy [ORCID]

  2. Author Address

    CICbioGUNE, Spain., University of Minnesota, United States., European Synchrotron Radiation Facility, France., Shubnikov Institute of Crystallography of FSRC, Crystallography and Photonics RAS, Russian Federation., University of Minnesota., Russian Academy of Sciences., Russian Academy of Sciences, Russian Federation., NCI RAS Initiative, Frederick National Laboratory for Cancer Research, Frederick, MD, USA, United States., Structural Biology Program, Memorial Sloan-Kettering Cancer Center, United States., The Hormel Institute, University of Minnesota, United States.,
    1. Year: 2018
    2. Date: Sep 11
    3. Epub Date: 2018 09 11
  2. Journal: Journal of Biological Chemistry
    1. Pages: pii: jbc.RA117.000733
  4. Type of Article: Article
  1. Abstract:

    The glycolipid transfer protein (GLTP) fold defines a superfamily of eukaryotic proteins that selectively transport sphingolipids (SLs) between membranes. Yet, the mechanisms determining the protein selectivity for specific glycosphingolipids (GSLs) are unclear. Here, we report the crystal structure of the GLTP-homology (GLTPH) domain of human 4 phosphate adaptor protein 2 (FAPP2) bound with N-oleoyl-galactosylceramide. Using this domain, FAPP2 transports glucosylceramide from its cis-Golgi synthesis site to the trans-Golgi for conversion into complex GSLs. The FAPP2-GLTPH structure revealed an element, termed the ID loop, that controls specificity in the GLTP family. We found that, in accordance with FAPP2 preference for simple GSLs, the ID loop protrudes from behind the SL headgroup-recognition center to mitigate binding by complex GSLs. Mutational analyses including GLTP and FAPP2 chimeras with swapped ID loops supported the proposed restrictive role of the FAPP2 ID loop in GSL selectivity. Comparative analysis revealed distinctly designed ID loops in each GLTP-family member. This analysis also disclosed a conserved H-bond triplet that "clasps" both ID-loop ends together to promote structural autonomy and rigidity. The findings indicated that various ID loops work in concert with conserved recognition centers to create different specificities among family members. We also observed four bulky, conserved hydrophobic residues involved in "sensor-like" interactions with lipid chains in protein hydrophobic pockets and FF-motifs in GLTP and FAPP2, well-positioned to provide acyl chain-dependent SL-selectivity for the hydro¬phobic pockets. In summary, our study provides mechanistic insights into sphingolipid recognition by the GLTP-fold and uncovers the elements involved in this recognition. Published under license by The American Society for Biochemistry and Molecular Biology, Inc.

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  2. DOI: 10.1074/jbc.RA117.000733
  3. PMID: 30206120
  4. PII : RA117.000733

Library Notes

  1. Fiscal Year: FY2017-2018
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