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ON-CHIP WEBINAR
October 2025

We are pleased to invite Rhea Bains from the University of British Columbia to present a webinar.
We will look at the discovery of novel N-glycan-degrading enzymes using droplet and the elucidation of the N-glycan degradation pathway!

Event Details

  • Date & Time: Wednesday, October 21 PST 2PM (EST 5PM)

  • Event Style: Zoom Webinar
    URL to enter the room will be sent to those who have registered.

  • Time Table:
    2:00 - 2:15 Introduction of Application notes
    #1 : Detection of Microbial Growth in Droplets Using Membrane Staining Reagents
    #2 :  Development of Substrates That Do Not Leak from Droplets
    #3 : A highly efficient bacteriophage screening method using water-in-oil droplet technology

    2:15 - 2:45 WEBINAR
    2:45 - 3:00 Q & A
名称未設定のデザイン-Sep-24-2025-05-04-03-2260-AM

Speaker

Rhea Bains
Phd student at the Univ. of British Columbia

Abstracts

Uncovering microbial N-glycan degradation pathways through ultrahigh-throughput single emulsion droplet screening.

Rajneesh K. Bains (1), Charlotte Olagnon (1), Jacob F. Wardman (1), Stephen G. Withers (1),
(1) Department of Chemistry, University of British Columbia, Vancouver, BC V6T 1Z3, Canada

N-glycans play a critical role within the human glycome. To advance our understanding of these glycans, it is essential to expand the current enzymatic Functional metagenomics offers a promising approach, significantly accelerating the discovery of novel enzymes, particularly glycoside However, a common challenge in such screenings is that the substrates used to identify target enzymes often fail to accurately represent those encountered in vivo. To address this limitation, our work focuses on designing substrates that better represent the structural complexity of glycans, using To address this limitation, our work focuses on designing substrates that better represent the structural complexity of glycans, using complex-type N-glycans as a proof of concept.

We have developed a novel fluorescence-quenched N-glycan probe that, when cleaved by enzymes capable of breaking any linkage within complex N-glycans, activates fluorescence. This enables the facile identification of genes encoding N-glycan-degrading enzymes. Our lab has also recently introduced a Our lab has also recently introduced a robust ultrahigh-throughput droplet-based platform that significantly accelerates the screening of metagenomic libraries. several advantages, including a significant reduction in the amount of substrate needed-particularly valuable when working with We have successfully integrated the fluorescence-quenched N We have successfully integrated the fluorescence-quenched N-glycan probe into this platform, enabling the screening of several metagenomic libraries to identify N-glycan-degrading pathways from diverse environments. Overall, our findings highlighting the power of ultrahigh-throughput screening platforms in discovering enzymes with the desired Overall, our findings highlighting the power of ultrahigh-throughput screening platforms in discovering enzymes with the desired activities and open new possibilities for developing probes that can identify such enzymes.

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What are DROPLETS ??

Microscopic water droplets dispersed in oil, stabilized by surfactants. Each droplet can encapsulate individual cells or microorganisms, creating millions of isolated micro-environments for parallel analysis.

app_droplet_image01_en (1)

ADVANTAGES

  •  Each droplet (picoliter-scale) functions as each well (microliter-scale) of a well-plate.
  •  Over one million droplets (reaction compartments) can be stored in a single tube.
  •  Significant savings can be achieved in analysis time, reagent consumption, and incubation space.
  •  Target droplet can be screened by On-chip Sort/On-chip Droplet Selector