Assembly of B4GALT1/ST6GAL1 heteromers in the Golgi membranes involves lateral interactions via highly charged surface domains.

β-1，4-Galactosyltransferase 1 (B4GALT1) and ST6 β-galactoside α-2，6-sialyltransferase 1 (ST6GAL1) catalyze the successive addition of terminal β-1，4-linked galactose and α-2，6-linked sialic acid to N-glycans. Their exclusive interaction in the Golgi compartment is a prerequisite for their full catalytic activity， whereas a lack of this interaction is associated with cancers and hypoxia. To date， no structural information exists that shows how glycosyltransferases functionally assemble with each other. Using molecular docking simulations to predict interaction surfaces， along with mutagenesis screens and high-throughput FRET analyses in live cells to validate these predictions， we show here that B4GALT1 and ST6GAL1 interact via highly charged non-catalytic surfaces， leaving the active sites exposed and accessible for donor and acceptor substrate binding. Moreover， we found that the assembly of ST6GAL1 homomers in the endoplasmic reticulum (ER) before ST6GAL1 activation in the Golgi utilizes the same non-catalytic surface， whereas B4GALT1 uses its active-site surface for assembly， which silences its catalytic activity. Lastly， we show that the homomeric and heteromeric B4GALT1/ST6GAL1 complexes can assemble laterally in the Golgi membranes without forming cross-cisternal contacts between enzyme molecules residing in the opposite membranes of each Golgi cisterna. Our results provide detailed mechanistic insights into the regulation of glycosyltransferase interactions， the transitions between B4GALT1 and ST6GAL1 homo- and heteromers in the Golgi， and cooperative B4GALT1/ST6GAL1 function in N-glycan synthesis.