Differential centrifugation


Differential centrifugation is a common procedure in biochemistry and cell biology used to separate organelles and other sub-cellular particles on the basis of sedimentation rate. Although often applied in biological analysis, differential centrifugation is a general technique also suitable for crude purification of non-living suspended particles. In a typical case where differential centrifugation is used to analyze cell-biological phenomena, a tissue sample is first lysed to break the cell membranes and release the organelles and cytosol. The lysate is then subjected to repeated centrifugations, where particles that sediment sufficiently quickly at a given centrifugation force for a given time form a compact "pellet" at the bottom of the centrifugation tube. After each centrifugation, the supernatant is removed from the tube and re-centrifuged at an increased centrifugal force and/or time. Differential centrifugation is suitable for crude separations on the basis of sedimintation rate, but more fine grained purifications may be done on the basis of density through equilibrium density-gradient centrifugation.

Theory

In a viscous fluid, the rate of sedimentation of a given suspended particle is largely a function of the particle size. Larger particles sediment more quickly and at lower centrifugal forces. If a particle is less dense than the fluid, the particle will not sediment, but rather will float, regardless of strength of the g-force experienced by the particle. In contrast, a more specialized equilibrium density-gradient centrifugation produces a separation profile dependent on particle-density alone, and therefore is suitable for more fine-grained separations.
High g-force makes sedimentation of small particles much faster than Brownian diffusion, even for very small particles. When a centrifuge is used, Stokes' law must be modified to account for the variation in g-force with distance from the center of rotation.
where
Differential centrifugation can be used with intact particles, or used to separate the component parts of a given particle. Using the example of a separation of eukaryotic organelles from intact cells, the cell must first be lysed and homogenized. Once the crude organelle extract is obtained, it may be subjected to a varying centrifugation speeds to separate the organelles:
Sample inputG forceTimeInstrument neededPellet contentsSupernatant contents
Unlysed cells100 x g5 minBenchtop fixed-angle centrifuge, or swinging bucket centrifugeIntact cells, macroscopic debrisVaries depending on sample
Gently lysed cells 600 x g10 minBenchtop fixed-angle centrifuge, or swinging bucket centrifugeNucleiCytosol, non-nuclei organelles
Supernatant of previous row15,000 x g20 minBenchtop fixed-angle centrifugeMitochondria, chloroplasts, lysosomes, peroxisomesCytosol, microsomes
Supernatant of previous row50,000 x g - 100,000 x g60 minHigh speed fixed-angle centrifuge, or vacuum ultracentrifugePlasma membrane, microsomal fraction, large polyribisomesCytosol, ribosomal subunits, small poly ribosomes, enzyme complexes
Supernatant of previous row50,000 x g - 100,000 x g120 minVacuum ultracentrifugeRibosomal subunits, small poly ribosomes, some soluble enzyme complexesCytosol

Ultracentrifugation

The lysed sample is now ready for centrifugation in an ultracentrifuge. An ultracentrifuge consists of a refrigerated, low-pressure chamber containing a rotor which is driven by an electrical motor capable of high speed rotation. Samples are placed in tubes within or attached to the rotor. Rotational speed may reach up to 100,000 rpm for floor model, 150,000 rpm for bench-top model, creating centrifugal speed forces of 800,000g to 1,000,000g. This force causes sedimentation of macromolecules, and can even cause non-uniform distributions of small molecules.
Since different fragments of a cell have different sizes and densities, each fragment will settle into a pellet with different minimum centrifugal forces. Thus, separation of the sample into different layers can be done by first centrifuging the original lysate under weak forces, removing the pellet, then exposing the subsequent supernatants to sequentially greater centrifugal fields. Each time a portion of different density is sedimented to the bottom of the container and extracted, and repeated application produces a rank of layers which includes different parts of the original sample. Additional steps can be taken to further refine each of the obtained pellets.
Sedimentation depends on mass, shape, and partial specific volume of a macromolecule, as well as solvent density, rotor size and rate of rotation. The sedimentation velocity can be monitored during the experiment to calculate molecular weight.
Values of sedimentation coefficient can be calculated. Large values of S correspond to larger molecular weight. Dense particle sediments more rapidly. Elongated proteins have larger frictional coefficients, and sediment more slowly to ensure accuracy.