Analytical ultracentrifugation
Analytical ultracentrifugation is an analytical technique which combines an ultracentrifuge with optical monitoring systems.
In an analytical ultracentrifuge (commonly abbreviated as AUC), a sample’s sedimentation profile is monitored in real time by an optical detection system. The sample is detected via ultraviolet light absorption and/or interference optical refractive index sensitive system, monitored by light-sensitive diode array or by film in the older machines. The operator can thus observe the change of sample concentration versus the axis of the rotation profile with time as a result of the applied centrifugal field. With modern instrumentation, these observations are electronically digitized and stored for further mathematical analysis.
The information that can be obtained from an analytical ultracentrifuge includes the gross shape of macromolecules, conformational changes in macromolecules, and size distributions of macromolecules. With AUC it is possible to gain information on the number and subunit stoichiometry of non-covalent complexes and equilibrium constants of macromolecules such as proteins, DNA, nanoparticles or other assemblies from different molecule classes. The simplest measurement to be obtained is the sedimentation coefficient, which depends upon the size of the molecules being sedimented. This is the ratio of a particle's sedimentation velocity to the applied acceleration causing the sedimentation.
Analytical ultracentrifugation has recently seen a rise in use because of increased ease of analysis with modern computers and the development of software, including a National Institutes of Health supported software package, SedFit.
History
[edit]Instrumentation
[edit]An analytical ultracentrifuge has a light source and optical detectors. To allow the light to pass through the analyte during the ultracentrifuge run, specialized cells are required which have to meet high optical standards as well as to resist the centrifugal forces. Each cell consists of a housing, two windows made from optically pure quartz glass, and a centrepiece with one or two sectors and filling holes for the sector(s), closed with a screw plug in the housing. These cell are placed into a rotor cavity with a continuous bore, with a collar at the bottom to retain the cell.
Theory
[edit]Types of experiments
[edit]By applying specific equipment and adapting measurement parameters several types of experiments can be performed. Most common AUC experiments are sedimentation velocity and sedimentation equilibrium experiments.
Sedimentation velocity
[edit]Sedimentation velocity experiments render the shape and molar mass of the analytes, as well as their size-distribution.[2] The size resolution of this method scales approximately with the square of the particle radii, and by adjusting the rotor speed of the experiment size-ranges from 100 Da to 10 GDa can be covered. Sedimentation velocity experiments can also be used to study reversible chemical equilibria between macromolecular species, by either monitoring the number and molar mass of macromolecular complexes, by gaining information about the complex composition from multi-signal analysis exploiting differences in each components spectroscopic signal, or by following the composition dependence of the sedimentation rates of the macromolecular system, as described in Gilbert-Jenkins theory.
The experiment aims to monitor the sedimentation behavior at a fixed angular speed.
Sedimentation equilibrium
[edit]Sedimentation equilibrium experiments reports the molar mass of analytes and their chemical equilibrium constants.[3] The rotor speed is adjusted such that a steady-state concentration profile c(r) of the sample in the cell is formed, where sedimentation and diffusion cancel out each other.
Density gradient centrifugation
[edit]Data evaluation
[edit]See also
[edit]- Ultracentrifuge
- Gas centrifuge
- Theodor Svedberg
- Differential centrifugation
- Buoyant density ultracentrifugation
- Zippe-type centrifuge
References
[edit]- ^ "Technical Manual, Spinco Ultracentrifuge Model E". Science History Institute Digital Collections. Retrieved 2018-12-18.
- ^ Perez-Ramirez, B. and Steckert, J.J. (2005). Therapeutic Proteins: Methods and Protocols. C.M. Smales and D.C. James, Eds. Volume 308: 301-318. Humana Press Inc, Totowa, NJ.
- ^ Ghirlando, R. (2011). "The analysis of macromolecular interactions by sedimentation equilibrium". Modern Analytical Ultracentrifugation: Methods. 58 (1): 145–156. doi:10.1016/j.ymeth.2010.12.005. PMC 3090454. PMID 21167941.
External links
[edit]- Reversible Associations in Structural and Molecular Biology (RASMB -an Analytical Ultracentrifugation Forum)
- Analytical Ultracentrifugation as a Contemporary Biomolecular Research Tool. Archived 2002-08-04 at the Wayback Machine
- Gilbert-Jenkins theory Archived 2007-05-01 at the Wayback Machine
- Report on an ultracentrifuge explosion.
Further reading
[edit]- Lebowitz J, Lewis MS, Schuck P (Jan 2005). "Modern analytical ultracentrifugation in protein science: A tutorial review". Protein Science. 102 (9): 2067–2069. doi:10.1110/ps.0207702. PMC 2373601. PMID 12192063.
- Balbo A, Minor KH, Velikovsky CA, Mariuzza RA, Peterson CB, Schuck P (Jan 2005). "Studying multiprotein complexes by multisignal sedimentation velocity analytical ultracentrifugation". PNAS. 102 (1): 81–86. Bibcode:2005PNAS..102...81B. doi:10.1073/pnas.0408399102. PMC 538923. PMID 15613487.
- Cole J, Hansen J (Dec 1999). "Analytical ultracentrifugation as a contemporary biomolecular research tool". J Biomol Tech. 10 (4): 163–76. PMC 2291609. PMID 19499023.