2005
DOI: 10.1016/j.gene.2005.05.042
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Perspectives for systematic in vitro antibody generation

Abstract: After the completion and refinement of the human genome, the characterization of individual gene products in respect of their functions, their modifications, their cellular localization and regulation in both space and time has generated an increased demand for antibodies for their analysis. Taking into account that the human genome contains¨25,000 genes, and that their products are found in different splice variants and produce proteins with post-translational modifications, it can be estimated that at least … Show more

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Cited by 68 publications
(45 citation statements)
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“…When trying to match the available funding with the task of generating more than 100,000 reagents, it becomes clear that new solutions and technical optimizations must be found. High-throughput approaches must be adopted at all levels, from protein expression and binder production to multiplexed assays and multiparameter tests 35 , and will be an integral part of any design of a binder-generation pipeline 36 .…”
Section: Linking Binders To Tools and Applicationsmentioning
confidence: 99%
“…When trying to match the available funding with the task of generating more than 100,000 reagents, it becomes clear that new solutions and technical optimizations must be found. High-throughput approaches must be adopted at all levels, from protein expression and binder production to multiplexed assays and multiparameter tests 35 , and will be an integral part of any design of a binder-generation pipeline 36 .…”
Section: Linking Binders To Tools and Applicationsmentioning
confidence: 99%
“…Second, antibody fragments can be displayed with increased efficiency on virions Rondot et al, 2001). Third, increased numbers of biopanned clones can be tested by robotic high throughput screening (de Wildt et al, 2000;Konthur et al, 2005).…”
Section: Introductionmentioning
confidence: 99%
“…Afterwards, these individual binders can be sequenced and further biochemically characterised (Hust et al, 2007a;Winter et al, 1994). This panning process can also be performed in a high-throughput manner (Buckler et al, 2008;Hallborn and Carlsson, 2002;Hust et al, 2011;Konthur et al, 2005). Because the gene sequence of the binder is available, the antibody -depending on the desired application -can be converted into different antibody formats (e.g.…”
Section: Antibody Phage Displaymentioning
confidence: 99%