Sequential affinity chromatography miniaturized within a “lab-on-valve” system

Erxleben, H.; Růžička, Jaromír

doi:10.1039/b501039j

Cited by 26 publications

(23 citation statements)

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“…Sepharose agarose beads were employed for affinity capture-release of biotincontaining conjugates with mass spectrometry (MS) detection [30]. Numerous biochemical applications have also been reported for the use of Protein A and Protein G Sepharose 4B conjugates [31][32][33]. Collagen-modified Cytodex 3 beads were used for non-covalent attachment of a phosphorescent oxygen probe (Pt-porphyrin complex) for detection of the oxygen consumption of adherent cell cultures [34].…”

Section: Solid Microparticles Used In Suspensions In Flow Analysismentioning

confidence: 99%

“…After measurement, the beads are removed by retracking the capillary or reversing the fluid flow. This design was used in SIA determinations of the oxygen consumption of cultured cells with fluorescence detection [33]. Two versions of the jet ring cell with radial and axial probing light paths have been developed and used in FIA measurements for bioligand interaction assays [29,42].…”

Section: Handling Suspensions Of Particles In Flow Systemsmentioning

confidence: 99%

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Application of Moveable Suspensions of Solid Particles in Flow Analysis

Trojanowicz

2008

Advances in Flow Analysis

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Section: Solid Microparticles Used In Suspensions In Flow Analysismentioning

confidence: 99%

Section: Handling Suspensions Of Particles In Flow Systemsmentioning

confidence: 99%

Application of Moveable Suspensions of Solid Particles in Flow Analysis

Trojanowicz

2008

Advances in Flow Analysis

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“…The microaffinity chromatography in the LOV format has been demonstrated for separation of immunoglobulins or nucleic acids, as based on molecular recognition between a site fixed on the stationary phase and the target species that is being captured, while unwanted matrix components, such as salts and proteins, are washed out by the mobile phase. In contrast to conventional immunoaffinity chromatography it is readily feasible to control the operational pH, which is a very critical parameter, and compared to on-column spectroscopy, LOV-chromatography on a renewable bead column is more robust, since the volume of the beads captured within the microcolumn is far less critical, and also because the target analyte is eluted and monitored in solution and not on bead surfaces, thus precluding light scattering effects (67,76). Furthermore, by using a short pulse of eluant, the front elution contains almost all target molecules, yielding excellent limits of detection.…”

Section: X72 Bioseparations and Cellular Assaysmentioning

confidence: 99%

“…7B). While the first approach can be viewed as "on-column spectroscopy" (15,74,75), the latter one can be considered as miniaturized bioaffinity chromatography (59,60,67). Both methods employ in-valve bead injection analysis with renewable microcolumns and identical analytical instrumentation, whereby they can be exploited in a complementary fashion to get further knowledge on biomolecular association and dissociation reactions (76,88).…”

Section: X72 Bioseparations and Cellular Assaysmentioning

confidence: 99%

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Flow Injection Analysis in Industrial Biotechnology

Hansen

Miró

2009

Encyclopedia of Industrial Biotechnology

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Flow injection analysis (FIA) is an analytical chemical continuous flow (CF) method which, in contrast to traditional CF procedures, does not rely on complete physical mixing (homogenization) of the sample and the reagent(s) or on attaining chemical equilibria of the chemical reactions involved. Exploiting controllable dispersion of the injected sample within the reagent‐containing carrier stream and strictly reproducible timing of all events taking place, it is based on measuring transient signals, which not only implies very high sampling rates but also, and most importantly, permits implementation of a number of novel methodologies that are not feasible when performed under batch conditions or by conventional CF procedures. Demonstrated for selected bioanalytical and technological applications encompassing cellular and enzymatic assays as well as monitoring of culture media, the principles and operational characteristics of FIA are first outlined, and then its downscaled/miniaturized sequels, that is, sequential injection analysis (SIA) and lab‐on‐valve (LOV), are detailed. Thus, in SIA the sample and reagents are, via the use of a multi‐position valve and an attached syringe pump operated under full programmable control, aspirated sequentially and then propelled forward allowing the sample and reagent(s) to be intermixed and, if called for, subjected to appropriate treatments before analyte detection. This infers that, merely minute sample/reagent volumes are consumed, hence leading to generation of small amounts of waste. In LOV this downscaling is taken further by using a small monolithic structure within which all sample manipulations and ultimate analyte detection under programmable control can be effected. Even bead materials with different surface groups/characteristics, including live cells, can be handled and utilized as demonstrated. Because the syringe pump in SIA and LOV can be used for accurately aspirating, propelling or even stopping the flow, these modi operandi allow fully to exploit the interplay between the kinetics and the thermodynamics of the chemical reactions involved, so that there are no restrictions whatsoever as to the chemistries that can be implemented, even if they entail multistep reactions. Representative bioanalytical examples of this interplay are presented.

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