Transglycanases(endotransglycosylases) cleave a polysaccharide(donor-substrate) in mid-chain, and then transfer a portion onto another poly-or oligosaccharide(acceptor-substrate). Such enzymes contribute to plan...Transglycanases(endotransglycosylases) cleave a polysaccharide(donor-substrate) in mid-chain, and then transfer a portion onto another poly-or oligosaccharide(acceptor-substrate). Such enzymes contribute to plant cellwall assembly and/or re-structuring. We sought a general method for revealing novel homo- and hetero-transglycanases, applicable to diverse polysaccharides and oligosaccharides, separating transglycanase-generated3 Hpolysaccharides from unreacted3H-oligosaccharides—the former immobilized(on filter-paper, silica-gel or glassfiber),the latter eluted. On filter-paper, certain polysaccharides [e.g.(1!3, 1!4)-b-D-glucans] remained satisfactorily adsorbed when water-washed; others(e.g. pectins) were partially lost. Many oligosaccharides(e.g. arabinan-, galactan-, xyloglucan-based) were successfully eluted in appropriate solvents, but others(e.g. [3H]xylohexaitol, [3H]mannohexaitol[3H]cellohexaitol) remained immobile. On silica-gel, all3 Holigosaccharides left an immobile ‘ghost’ spot(contaminating any3H-polysaccharides), which was diminished but not prevented by additives e.g. sucrose or Triton X-100. The best stratum was glassfiber(GF), onto which the reactionmixture was dried then washed in 75% ethanol. Washing led to minimal loss or lateral migration of3H-polysaccharides if conducted by slow percolation of acidified ethanol. The effectiveness of GF-blotting was well demonstrated for Chara vulgaris transb-mannanase. In conclusion, our novel GF-blotting technique ef ficiently frees transglycanase-generated3H-polysaccharides from unreacted3H-oligosaccharides,enabling high-throughput screening of multiple postulated transglycanase activities utilising chemically diverse donorand acceptor-substrates.展开更多
基金the Leverhulme Foundation (sponsor reference F00158/CI)
文摘Transglycanases(endotransglycosylases) cleave a polysaccharide(donor-substrate) in mid-chain, and then transfer a portion onto another poly-or oligosaccharide(acceptor-substrate). Such enzymes contribute to plant cellwall assembly and/or re-structuring. We sought a general method for revealing novel homo- and hetero-transglycanases, applicable to diverse polysaccharides and oligosaccharides, separating transglycanase-generated3 Hpolysaccharides from unreacted3H-oligosaccharides—the former immobilized(on filter-paper, silica-gel or glassfiber),the latter eluted. On filter-paper, certain polysaccharides [e.g.(1!3, 1!4)-b-D-glucans] remained satisfactorily adsorbed when water-washed; others(e.g. pectins) were partially lost. Many oligosaccharides(e.g. arabinan-, galactan-, xyloglucan-based) were successfully eluted in appropriate solvents, but others(e.g. [3H]xylohexaitol, [3H]mannohexaitol[3H]cellohexaitol) remained immobile. On silica-gel, all3 Holigosaccharides left an immobile ‘ghost’ spot(contaminating any3H-polysaccharides), which was diminished but not prevented by additives e.g. sucrose or Triton X-100. The best stratum was glassfiber(GF), onto which the reactionmixture was dried then washed in 75% ethanol. Washing led to minimal loss or lateral migration of3H-polysaccharides if conducted by slow percolation of acidified ethanol. The effectiveness of GF-blotting was well demonstrated for Chara vulgaris transb-mannanase. In conclusion, our novel GF-blotting technique ef ficiently frees transglycanase-generated3H-polysaccharides from unreacted3H-oligosaccharides,enabling high-throughput screening of multiple postulated transglycanase activities utilising chemically diverse donorand acceptor-substrates.
