Literature DB >> 9249148

A lectin method for investigating the glycosylation of nanogram amounts of purified glycoprotein.

M T Goodarzi1, G A Turner.   

Abstract

To unravel the complexities of the glycosylation of a protein is a substantial task, which requires considerable effort and resources. However, in many situations this is unnecessary, because only a limited amount of information is required. A new lectin-binding assay is described which is rapid, cheap and versatile. A purified glycoprotein is absorbed on to the plastic surface of a microtitre plate. After removing unbound protein by washing, uncoated sites on the plate are blocked and digoxigenin or biotin-labelled lectin is added. The degree of lectin binding is measured using either an anti-DIG antibody or streptavidin conjugated enzyme, which is subsequently used to develop a colour reaction. Using this method it is possible to screen multiple specimens with high sensitivity and excellent precision. In addition, very small amounts of lectin are used, background absorbances are low, and the procedure does not require a high degree of technical skill. Because very small amounts of glycoprotein are needed, a glycoprotein can often be rapidly purified by batch affinity chromatography. The method has been successfully applied to several purified proteins using the lectins, Con A, LCA, LTA, MAA, and SNA, and the information obtained agrees with that produced by more sophisticated approaches, eg Dionex Carbohydrate Analyser. Using a panel of lectins, a carbohydrate structural profile is quickly built-up, and subtle differences in glycosylation identified. This method should be particularly useful for screening glycosylation in multiple clinical specimens; in specimens where very small amounts of material are available, such as membrane molecules; and in the screening of recombinant proteins produced commercially.

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Year:  1997        PMID: 9249148     DOI: 10.1023/a:1018507703589

Source DB:  PubMed          Journal:  Glycoconj J        ISSN: 0282-0080            Impact factor:   2.916


  7 in total

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Journal:  Eur J Biochem       Date:  1992-10-15

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Authors:  G A Turner
Journal:  Clin Chim Acta       Date:  1992-06-30       Impact factor: 3.786

3.  An improved multiwell immunoassay using digoxigenin-labelled lectins to study the glycosylation of purified glycoproteins.

Authors:  M T Goodarzi; M Rafiq; G Turner
Journal:  Biochem Soc Trans       Date:  1995-05       Impact factor: 5.407

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Authors:  T W Rademacher; R B Parekh; R A Dwek
Journal:  Annu Rev Biochem       Date:  1988       Impact factor: 23.643

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Authors:  G A Turner; M T Goodarzi; S Thompson
Journal:  Glycoconj J       Date:  1995-06       Impact factor: 2.916

6.  Decreased branching, increased fucosylation and changed sialylation of alpha-1-proteinase inhibitor in breast and ovarian cancer.

Authors:  M T Goodarzi; G A Turner
Journal:  Clin Chim Acta       Date:  1995-05-15       Impact factor: 3.786

Review 7.  The oligosaccharides of glycoproteins: bioprocess factors affecting oligosaccharide structure and their effect on glycoprotein properties.

Authors:  C F Goochee; M J Gramer; D C Andersen; J B Bahr; J R Rasmussen
Journal:  Biotechnology (N Y)       Date:  1991-12
  7 in total
  6 in total

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Authors:  Marta Piva; J Ignacio Moreno; Kathy L Sharpe-Timms
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2.  Lectin binding assays for in-process monitoring of sialylation in protein production.

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Review 4.  Carbohydrate recognition by boronolectins, small molecules, and lectins.

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Review 5.  Lectins as tools in glycoconjugate research.

Authors:  Albert M Wu; Elwira Lisowska; Maria Duk; Zhangung Yang
Journal:  Glycoconj J       Date:  2009-11       Impact factor: 2.916

6.  Identification of aberrantly expressed glycans in gastric cancer by integrated lectin microarray and mass spectrometric analyses.

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  6 in total

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