In vivo activities of heparan sulfate differentially modified by NDSTs during development

Author:

Nakato Eriko1,Baker Sarah1,Kinoshita‐Toyoda Akiko2,Knudsen Collin1ORCID,Lu Yi‐Si1,Takemura Masahiko1,Toyoda Hidenao2,Nakato Hiroshi1

Affiliation:

1. Department of Genetics, Cell Biology, and Development University of Minnesota Minneapolis Minnesota USA

2. Faculty of Pharmaceutical Sciences Ritsumeikan University Shiga Japan

Abstract

AbstractHeparan sulfate proteoglycans (HSPGs) serve as co‐receptors for growth factor signaling during development. It is well known that the level and patterns of sulfate groups of heparan sulfate (HS) chains, or HS fine structures, have a major impact on HSPG function. On the other hand, the physiological significance of other structural features of HS, including NS/NA domain organization, remains to be elucidated. A blueprint of the HS domain structures is mainly controlled by HS N‐deacetylase/N‐sulfotransferases (NDSTs). To analyze in vivo activities of differentially modified HS, we established two knock‐in (KI) Drosophila strains with the insertion of mouse Ndst1 (mNdst1) or Ndst2 (mNdst2) in the locus of sulfateless (sfl), the only Drosophila NDST. In these KI lines, mNDSTs are expressed from the sfl locus, in the level and patterns identical to the endogenous sfl gene. Thus, phenotypes of Ndst1 KI and Ndst2KI animals reflect the ability of HS structures made by these enzymes to rescue sfl mutation. Remarkably, we found that mNdst1 completely rescued the loss of sfl. mNdst2 showed a limited rescue ability, despite a higher level of HS sulfation compared to HS in mNdst1 KI. Our study suggests that independent of sulfation levels, additional HS structural features controlled by NDSTs play key roles during tissue patterning.

Funder

National Institutes of Health

Publisher

Wiley

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