Nesterenko AM et al. (2015), Affinity of the heparin binding motif of Noggin...

XB-ART-51528

Biochem Biophys Res Commun 2015 Dec 04;4681-2:331-6. doi: 10.1016/j.bbrc.2015.10.100.

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Affinity of the heparin binding motif of Noggin1 to heparan sulfate and its visualization in the embryonic tissues.

Nesterenko AM , Orlov EE , Ermakova GV , Ivanov IA , Semenyuk PI , Orlov VN , Martynova NY , Zaraisky AG .

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Heparin binding motifs were found in many secreted proteins and it was suggested that they are responsible for retardation of the protein diffusion within the intercellular space due to the binding to heparan sulfate proteoglycanes (HSPG). Here we used synthetic FITC labeled heparin binding motif (HBM peptide) of the Xenopus laevis secreted BMP inhibitor Noggin1 to study its diffusion along the surface of the heparin beads by FRAP method. As a result, we have found out that diffusivity of HBM-labeled FITC was indeed much lesser than those predicted by theoretical calculations even for whole protein of the Noggin size. We also compared by isothermal titration calorimetry the binding affinity of HBM and the control oligolysine peptide to several natural polyanions including heparan sulfate (HS), heparin, the bacterial dextran sulfate and salmon sperm DNA, and demonstrated that HBM significantly exceeds oligolysine peptide in the affinity to HS, heparin and DNA. By contrast, oligolysine peptide bound with higher affinity to dextran sulfate. We speculate that such a difference may ensure specificity of the morphogen binding to HSPG and could be explained by steric constrains imposed by different distribution of the negative charges along a given polymeric molecule. Finally, by using EGFP-HBM recombinant protein we have visualized the natural pattern of the Noggin1 binding sites within the X. laevis gastrula and demonstrated that these sites forms a dorsal-ventral concentration gradient, with a maximum in the dorsal blastopore lip. In sum, our data provide a quantitative basis for modeling the process of Noggin1 diffusion in embryonic tissues, considering its interaction with HSPG.

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Species referenced: Xenopus laevis
Genes referenced: bcr lrp5 mcf2 mtor nog sdc2

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	graphical abstract
	Fig. 1. In vitro and theoretical FRAP. (a) Recovery kinetics normalized to mobile fraction of HBM-FITC in vitro (points); all theoretical curves are plotted by Soumpasis equation. * – the green curve reflects predicted fluorescence recovery for free Noggin1 protein. ** – the blue curve is plotted according to in vivo measurements of Noggin1 diffusion [7] (see Materials & Methods for calculation details). (b,c) The confocal images of FRAP procedure: the bead before and after the bleaching. The white square marks the area of signal measurement. (d) Schematic of the in vitro FRAP experimental system. (For interpretation of the references to colour in this figure legend, the reader is referred to the web version of this article.)
	Fig. 2. Binding curves of ITC data. Oligolysine (blue, marked “OL”) and HBM peptide (black) were titrated into LMW heparin (a), heparan sulfate (b), dextran sulfate (c) and salmon sperm DNA (d). Calculated dissociation constants are presented on figures. Theoretical curves were plotted by using the model with equal independent binding sites. (For interpretation of the references to colour in this figure legend, the reader is referred to the web version of this article.)
	Fig. 3. Vibratome sections of Xenopus laevis embryo at midgastrula stage dyed with HBM-EGFP protein. (a) Sagittal section. Animal pole to the top, dorsal side to the right. (b) Large view of the dorsal blastopore lip; some dyed nuclei are indicated by arrowheads. Abbreviations: bcr – blastocoel roof; bcl – blastocoel; arch – invagination of archaenteron; dbl – dorsal blastopore lip; vbl – ventral blastopore lip; ypg – yolk plug; bot – bottle cells; bp – blastopore.