Margo D.M. de Jong scite author profile

Saccharomyces cerevisiae is often used to produce heterologous proteins that are preferentially secreted to increase economic feasibility. We used N-glycosylation as a tool to enhance protein secretion. Secretion of cutinase, a lipase, and llama V HH antibody fragments by S. cerevisiae or Pichia pastoris improved following the introduction of an N-glycosylation site. When we introduced an N-glycosylation consensus sequence in the N-terminal region of a hydrophobic cutinase, secretion increased fivefold. If an N-glycosylation site was introduced in the C-terminal region, however, secretion increased only 1.8-fold. These results indicate that the use of N glycosylation can significantly enhance heterologous protein secretion.

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Pre-embedding immunolabeling for electron microscopy: An evaluation of permeabilization methods and markers

Humbel

Jong

Müller

et al. 1998

Microsc. Res. Tech.

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Pre‐embedding immunolabeling for electron microscopy: An evaluation of permeabilization methods and markers

Humbel

Jong

Müller

et al. 1998

Microsc. Res. Tech.

View full text Add to dashboard Cite

For scarce antigens or antigens which are embedded in a dense macromolecular structure, on-section labeling, the first method of choice, is not always successful. Often, the antigen can be localized by immunofluorescence microscopy, usually by a pre-embedding labeling method. Most of these methods lead to loss of ultrastructural details and, hence, labeling at electron microscope resolution does not add essential information. The scope of this paper is to compare five permeabilization methods for pre-embedding labelling for electron microscopy. We aim for a method that is easy to use and suitable for routine investigations. For our ongoing work, special attention is given to labeling of the cell nucleus. Accessibility of cytoplasmic and nuclear antigens is monitored with a set of different marker antibodies. From this investigation, we suggest that prefixation with formaldehyde/glutaraldehyde is necessary to stabilize the ultrastructure before using a detergent (Triton X-100 or Brij 58) to permeabilize or remove the membranes. The experimental conditions for labeling should be checked first with fluorescence or fluorescence-gold markers by fluorescence microscopy. Then either ultrasmall gold particles (with or without fluorochrome) with silver enhancement or, if the ultrasmall gold particles are obstructed, peroxidase markers are advised. The most promising technique to localize scarce antigens with good contrast is the combination of a pre-embedding peroxidase/tyramide-FITC or -biotin labeling followed by an on-section colloidal gold detection.

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The taxonomic position of Asterodon, Asterostroma and Coltricia inferred from the septal pore cap ultrastructure

Müller

Stalpers

Aelst

et al. 2000

Mycological Research

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Margo D.M. de Jong

Introduction of an N-Glycosylation Site Increases Secretion of Heterologous Proteins in Yeasts

Pre-embedding immunolabeling for electron microscopy: An evaluation of permeabilization methods and markers

Pre‐embedding immunolabeling for electron microscopy: An evaluation of permeabilization methods and markers

The taxonomic position of Asterodon, Asterostroma and Coltricia inferred from the septal pore cap ultrastructure

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