Ccl19 With Ccl21-Tail Displays Enhanced Glycosaminoglycan Binding With Retained Chemotactic Potency In Dendritic Cells

JOURNAL OF LEUKOCYTE BIOLOGY(2018)

Cited 17|Views25
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Abstract
CCL19 is more potent than CCL21 in inducing chemotaxis of human dendritic cells (DC). This difference is attributed to 1) a stronger interaction of the basic C-terminal tail of CCL21 with acidic glycosaminoglycans (GAGs) in the environment and 2) an autoinhibitory function of this C-terminal tail. Moreover, different receptor docking modes and tissue expression patterns of CCL19 and CCL21 contribute to fine-tuned control of CCR7 signaling. Here, we investigate the effect of the tail of CCL21 on chemokine binding to GAGs and on CCR7 activation. We show that transfer of CCL21-tail to CCL19 (CCL19(CCL21-tail)) markedly increases binding of CCL19 to human dendritic cell surfaces, without impairing CCL19-induced intracellular calcium release or DC chemotaxis, although it causes reduced CCR7 internalization. The more potent chemotaxis induced by CCL19 and CCL19(CCL21-tail) compared to CCL21 is not transferred to CCL21 by replacing its N-terminus with that of CCL19 (CCL21(CCL19-N-term)). Measurements of cAMP production in CHO cells uncover that CCL21-tail transfer (CCL19(CCL21-tail)) negatively affects CCL19 potency, whereas removal of CCL21-tail (CCL21(tailless)) increases signaling compared to full-length CCL21, indicating that the tail negatively affects signaling via cAMP. Similar to chemokine-driven calcium mobilization and chemotaxis, the potency of CCL21 in cAMP is not improved by transfer of the CCL19 N-terminus to CCL21 (CCL21(CCL19-N-term)). Together these results indicate that ligands containing CCL21 core and C-terminal tail (CCL21 and CCL21(CCL19-N-term)) are most restricted in their cAMP signaling; a phenotype attributed to a stronger GAG binding of CCL21 and defined structural differences between CCL19 and CCL21.
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Key words
bias signaling, cAMP, chimera, migration, species bias, tail truncation
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