Introduction

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Literaturreferenz^[1]

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Introduction

Purpose

Any cell mesh produced based on our bioink will suffer from exposition to serum-containing media or, in the case of in vivo application, the patient’s body fluids because of biotinidase. This ubiquitous enzyme is able to cleave biotin off of lysine – at a lower rate also off of intact protein. We may now shift this hydrolysis in two directions: either to prevent it altogether and thus stabilize our cell mesh, or to accelerate it to make our mesh quickly disintegrable. To this end, we must consider how biotin is linked to the proteins in our bioink.

NHS Esters as Amine Coupling Reagents

Design

Experiments

Proof of concept

Demonstrate

Discussion

References

↑ Schmidt, T. G., & Skerra, A. (2007). The Strep-tag system for one-step purification and high-affinity detection or capturing of proteins. Nature protocols, 2(6), 1528-1535.

[1] Schmidt, T. G., & Skerra, A. (2007). The Strep-tag system for one-step purification and high-affinity detection or capturing of proteins. Nature protocols, 2(6), 1528-1535.

[1]

Team:LMU-TUM Munich/Linkerchemistry

Introduction

Kopiervorlagen

References

Textformatierung

Links

Bilder

Introduction

Purpose

NHS Esters as Amine Coupling Reagents

Design

Experiments

Proof of concept

Demonstrate

Discussion

References