Abstract
BackgroundSialyltransferases (SIATs) are a family of enzymes that transfer sialic acid (Sia) to glycan chains on glycoproteins, glycolipids, and oligosaccharides. They play key roles in determining cell–cell and cell-matrix interactions and are important in neuronal development, immune regulation, protein stability and clearance. Most fully characterized SIATs are of mammalian origin and these have been used for in vitro and in vivo modification of glycans. Additional versatility could be achieved by the use of animal SIATs from other species that live in much more variable environments. Our aim was to generate a panel of stable CHO cell lines expressing a range of vertebrate SIATs with different physicochemical and functional properties.MethodsThe soluble forms of various animal ST6Gal and ST3Gal enzymes were stably expressed from a Gateway-modified secretion vector in CHO cells. The secreted proteins were IMAC-purified from serum-free media. Functionality of the protein was initially assessed by lectin binding to the host CHO cells. Activity of purified proteins was determined by a number of approaches that included a phosphate-linked sialyltransferase assay, HILIC-HPLC identification of sialyllactose products and enzyme-linked lectin assay (ELLA).ResultsA range of sialyltransferase from mammals, birds and fish were stably expressed in CHO Flp-In cells. The stable cell lines expressing ST6Gal1 modify the glycans on the surface of the CHO cells as detected by fluorescently labelled lectin microscopy. The catalytic domains, as isolated by Ni Sepharose from culture media, have enzymatic activities comparable to commercial enzymes. Sialyllactoses were identified by HILIC-HPLC on incubation of the enzymes from lactose or whey permeate. The enzymes also increased SNA-I labelling of asialofetuin when incubated in a plate format.ConclusionStable cell lines are available that may provide options for the in vivo sialylation of glycoproteins. Proteins are active and should display a variety of biological and physicochemical properties based on the animal source of the enzyme.
Highlights
Sialyltransferases (SIATs) transfer sialic acid (Sia) to glycan chains on glycoproteins and glycolipids
Our focus in this study was on expressing the catalytic domains of the SIATs, for comparative purposes we constructed two full-length ST6Gal I expressing vectors
All catalytic domain-expressing constructs were based on pSecTag/FLP Recombination Target (FRT)/V5-His TOPO with inserts amplified by PCR from cDNA
Summary
Sialyltransferases (SIATs) transfer sialic acid (Sia) to glycan chains on glycoproteins and glycolipids. These sialylated structures are terminal structures on external cell surfaces they are key players in cell–cell, cell-pathogen and cell-matrix interactions, and are important factors in protein stability and clearance (Bragonzi et al, 2000; Choi et al, 2015; Olufsen, Brandsdal & Smalas, 2007), neuronal development (Galuska et al, 2006), and immune regulation (Hennet et al, 1998; Varki, 1999). Sialyltransferases (SIATs) are a family of enzymes that transfer sialic acid (Sia) to glycan chains on glycoproteins, glycolipids, and oligosaccharides. They play key roles in determining cell–cell and cell-matrix interactions and are important in neuronal development, immune regulation, protein stability and clearance. Proteins are active and should display a variety of biological and physicochemical properties based on the animal source of the enzyme
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