Highly Selective Separations in Biotechnology
Editat de G. Streeten Limba Engleză Paperback – 25 sep 2012
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Specificații
ISBN-13: 9789401045766
ISBN-10: 9401045763
Pagini: 248
Ilustrații: XII, 231 p.
Dimensiuni: 155 x 235 x 14 mm
Greutate: 0.38 kg
Ediția:Softcover reprint of the original 1st ed. 1994
Editura: Springer
Locul publicării:Dordrecht, Netherlands
ISBN-10: 9401045763
Pagini: 248
Ilustrații: XII, 231 p.
Dimensiuni: 155 x 235 x 14 mm
Greutate: 0.38 kg
Ediția:Softcover reprint of the original 1st ed. 1994
Editura: Springer
Locul publicării:Dordrecht, Netherlands
Public țintă
ResearchCuprins
1 Overview.- References.- 2 Affinity precipitation.- 2.1 Introduction.- 2.2 Various formats of affinity precipitation.- 2.3 Heterobifunctional ligands.- 2.4 Use of macro affinity ligands.- 2.5 Practical applications of affinity precipitation.- 2.6 Affinity precipitation by heterobifunctional ligands.- 2.7 Comparison of affinity precipitation with other affinity techniques.- 2.8 Conclusions.- References.- 3 Membrane-based affinity separation processes.- 3.1 Introduction.- 3.2 Chemical and physical feature of the membrane matrix.- 3.3 Purification protocol.- 3.4 Ligand coupling.- 3.5. Stability of active membranes.- 3.6 Reuse of ligand coupled membranes.- 3.7 Storage of ligand coupled membranes in buffer.- 3.8 Ligand leaching.- 3.9 Efficiency of ligand coupling.- 3.10 Effect of flow rates on affinity purification of IgG.- 3.11 Exhaustive purification of antibodies.- 3.12 Effect of sample recirculation on yields.- 3.13 Purification of IgG from ascites fluid and serum.- 3.14 Efficiency in product recovery.- 3.15 Applications.- 3.16 Scale-up.- 3.17 Discussion.- References.- 4 Affinity partitioning.- 4.1 Introduction.- 4.2 Two-phase systems.- 4.3 General ways of steering the partitioning.- 4.4 Affinity partitioning.- 4.5 Large-scale extractions.- 4.6 Use of two-phase systems in bioreactors.- 4.7 Non-protein partitioning.- 4.8 Alternative types of affinity ligands.- 4.9 Counter-current distribution.- 4.10 Conclusions.- References.- 5 The use of reverse micelles for the separation of proteins.- 5.1 Introduction.- 5.2 Description of reverse micelles.- 5.3 The reverse micellar extraction method.- 5.4 Protein distribution between an aqueous and a conjugated reverse micellar phase.- 5.5 Mass transfer of protein extraction.- 5.6 Process development.- 5.7 Examples of reverse micellarapplications for protein separation.- 5.8 Conclusions.- References.- 6 The chemistry and engineering of affinity chromatography.- 6.1 Introduction.- 6.2 The role of AC in protein purification.- 6.3 Affinity packings.- 6.4 Characterization of AC packings.- 6.5 Modelling and design of affinity chromatography columns.- 6.6 Notation.- References.- 7 Protein fusions as an aid to purification.- 7.1 Introduction.- 7.2 Choice of host organism.- 7.3 Induction of expression.- 7.4 Solubilisation of recombinant proteins.- 7.5 Vectors.- 7.6 Affinity purification.- 7.7 Thrombin cleavage of fusion proteins.- 7.8 General discussion.- References.- 8 Chiral separations.- 8.1 Introduction.- 8.2 Some stereochemical terms.- 8.3 Chirality and biological systems.- 8.4 Methods available for chiral separation.- 8.5 Conclusion.- References.- 9 Molecular imprinting—a versatile technique for the preparation of separation materials of predetermined selectivity.- 9.1 Introduction.- 9.2 Preparation of molecular imprints.- 9.3 Recognition in molecularly imprinted polymers.- 9.4 Application.- 9.5 Conclusions.- References.
Recenzii
Each chapter is well written, and provides a sound background understanding together with useful practical details and user experience ... It is a good source of ideas and solutions that will enable many to develop their own highly selective bioseparations. - The Genetic Engineer and Biotechnologist; This is a well put-together and presented book - highly practical in nature...Four stars. - Australian Biotechnology Association