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Fractionation of organelles and membrane vesicles using OptiPrep ™. Competitive products are sucrose and Percoll ® Sucrose-based publications go back to 1948. Golgi. Exocytosis/secretion. Caveolae. Trans-Golgi network. Lipid rafts. ERGIC. Coated pits. Endocytosis. N. Endocytic
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1. Fractionation of organelles and membrane vesicles using OptiPrep Competitive products are sucrose and Percoll
Sucrose-based publications go back to 1948 The vast number of publications reporting the use of sucrose gradients for the fractionation of subcellular particles makes a change to OptiPrep often quite difficult, but there are some important advantages in using OptiPrep. The vast number of publications reporting the use of sucrose gradients for the fractionation of subcellular particles makes a change to OptiPrep often quite difficult, but there are some important advantages in using OptiPrep.
2. The huge number of subcellular membrane compartments underscores the complexity of the task to produce pure preparations of any one type of particle or the development of gradients that will allow identification of multiple particle types. This short training file will therefore deal principally with some general points about subcellular fractionation; describe a few of the commonly used organelle isolation methods and end with a few examples of analyses that demonstrate the resolving power of iodixanol gradients in studies of membrane trafficking and cell signalling. The next series of slides however (Slides 3-9) describe in general terms the operations that are carried out and some of the requirements and consequences of these operations. The huge number of subcellular membrane compartments underscores the complexity of the task to produce pure preparations of any one type of particle or the development of gradients that will allow identification of multiple particle types. This short training file will therefore deal principally with some general points about subcellular fractionation; describe a few of the commonly used organelle isolation methods and end with a few examples of analyses that demonstrate the resolving power of iodixanol gradients in studies of membrane trafficking and cell signalling. The next series of slides however (Slides 3-9) describe in general terms the operations that are carried out and some of the requirements and consequences of these operations.
3. Iodixanol gradient solution strategy (S01, S02) Simple gradient solution preparation
When OptiPrep is diluted with the homogenization medium the solutions will be iso-osmotic Step 1 is solution preparation. The use of OptiPrep makes gradient solution preparation as easy as possible it may be simply diluted with a normal iso-osmotic tissue or cell homogenization medium and all the solutions produced will also be iso-osmotic. Step 1 is solution preparation. The use of OptiPrep makes gradient solution preparation as easy as possible it may be simply diluted with a normal iso-osmotic tissue or cell homogenization medium and all the solutions produced will also be iso-osmotic.
4. Percoll solution strategy Because Percoll has nearly zero osmolality the working solution must be made by diluting 9 vol of Percoll with 1 vol of 2.5 M sucrose
2.5 M sucrose is close to saturation
2.5 M sucrose is impossible to handle accurately Handling of Percoll is by contrast very difficult. Since Percoll has essentially no osmotic pressure, it is necessary first to produce a working solution by diluting 9 vol. with 1 vol. of 2.5 M sucrose. Firstly 2.5 M sucrose is difficult to prepare since it is close to saturation and it is so viscous that accurate volume dispensing is almost impossible.Handling of Percoll is by contrast very difficult. Since Percoll has essentially no osmotic pressure, it is necessary first to produce a working solution by diluting 9 vol. with 1 vol. of 2.5 M sucrose. Firstly 2.5 M sucrose is difficult to prepare since it is close to saturation and it is so viscous that accurate volume dispensing is almost impossible.
5. Differential centrifugation of homogenate Step 2 is differential centrifugation of the homogenate. The slide shows a widely used protocol that precedes any gradient. Sometimes an additional step is inserted in which the first 1000 g is centrifuged at 3000 g for 10 min to produce the so-called heavy mitochondrial fraction (HMF). This supernatant is then centrifuged at 15,000 g to produce the light mitochondrial fraction (LMF).
In the analysis of ER, Golgi and plasma membrane, some workers will first prepare a microsome fraction as described in the slide, but some people will simply use the first 1000 g supernatant. The latter will contain microsomes plus all the mitochondria, lysosomes and peroxisomes. Step 2 is differential centrifugation of the homogenate. The slide shows a widely used protocol that precedes any gradient. Sometimes an additional step is inserted in which the first 1000 g is centrifuged at 3000 g for 10 min to produce the so-called heavy mitochondrial fraction (HMF). This supernatant is then centrifuged at 15,000 g to produce the light mitochondrial fraction (LMF).
In the analysis of ER, Golgi and plasma membrane, some workers will first prepare a microsome fraction as described in the slide, but some people will simply use the first 1000 g supernatant. The latter will contain microsomes plus all the mitochondria, lysosomes and peroxisomes.
6. Carry out the density gradient centrifugation Suspend the relevant pellet in a small volume of homogenization buffer (or dense solution)
Layer the suspension on top of (or below) the gradient
Centrifuge usually in a swinging-bucket rotor
Collect the gradient in a series of fractions if required Step 3 Following some form of differential centrifugation, the selected fraction is then applied to a gradient and in most cases, but particularly in membrane trafficking and cell signalling studies, the gradient will be collected in a series of equal volume fractions and analyzedStep 3 Following some form of differential centrifugation, the selected fraction is then applied to a gradient and in most cases, but particularly in membrane trafficking and cell signalling studies, the gradient will be collected in a series of equal volume fractions and analyzed
7. Analyze fractions 20-30 fractions (0.5-1.0 ml each) need to be analyzed for some functional marker characteristic of each membrane and for total protein. Determine density of blank gradient
Measure marker enzyme spectrophotometrically OR do SDS-PAGE, electroblot and probe the blot with antibodies to marker proteins Step 4 is analysis of the gradient fractions.Step 4 is analysis of the gradient fractions.
8. Density gradient medium should not interfere with analysis I Percoll is light scattering at all wavelengths so must be removed prior to spectrophotometric analysis
Percoll must be removed prior to SDS-PAGE because it affects sample entry into gel
Removal of Percoll particles leads to loss of organelles Analysis of the fractions from a Percoll gradient pose important problems. The removal of Percoll means that each fraction is diluted and then centrifuged so that the Percoll particles form a pellet. The problem is that the g-force required to pellet the Percoll also causes the subcellular membranes to pellet as a result significant losses of cellular material can be incurred.Analysis of the fractions from a Percoll gradient pose important problems. The removal of Percoll means that each fraction is diluted and then centrifuged so that the Percoll particles form a pellet. The problem is that the g-force required to pellet the Percoll also causes the subcellular membranes to pellet as a result significant losses of cellular material can be incurred.
9. Only for spectrophotometric analysis in the UV must iodixanol (or Nycodenz) be removed
Removal of iodixanol (or Nycodenz) does not lead to loss of organelles
Sucrose need not be removed prior to any analysis Density gradient medium should not interfere with analysis II In the great majority of cases none of these problems apply to gradients of Nycodenz or iodixanol or sucrose. All of these are true solutes and if necessary the membranes can be simply be pelleted from each gradient solution after dilution. In the great majority of cases none of these problems apply to gradients of Nycodenz or iodixanol or sucrose. All of these are true solutes and if necessary the membranes can be simply be pelleted from each gradient solution after dilution.
10. Four important examples of simple discontinuous iodixanol gradients Purification of nuclei from a total homogenate
Purification of mitochondria from a crude mitochondrial fraction
Separation of cytosol and membrane vesicles
Isolation of lipid rafts The methodology is so extensive and various that it is not feasible to cover more than a few specimen isolations in any detail four of the most widely used fractionations are presented.The methodology is so extensive and various that it is not feasible to cover more than a few specimen isolations in any detail four of the most widely used fractionations are presented.
11. Purification of nuclei I (S08) A prime example of the advantages of an iodixanol separation over a sucrose one is the isolation of nuclei. In this rapid and organelle-friendly method the whole tissue or cell homogenate is simply mixed with OptiPrep (3.5:2.5 v/v) and layered over two solutions of 30% and 35% iodixanol. Under very mild centrifugation conditions the nuclei band at the lower interface. A prime example of the advantages of an iodixanol separation over a sucrose one is the isolation of nuclei. In this rapid and organelle-friendly method the whole tissue or cell homogenate is simply mixed with OptiPrep (3.5:2.5 v/v) and layered over two solutions of 30% and 35% iodixanol. Under very mild centrifugation conditions the nuclei band at the lower interface.
12. Purification of nuclei II Advantages over sucrose
Density barriers of 60-65% sucrose - very difficult to prepare
Sucrose solutions very viscous, therefore need much higher g-forces (100-150,000g and times (1-2 h)
Sucrose solutions are vastly hyperosmotic; only iodixanol allows nuclear isolation under iso-osmotic conditions
Iodixanol method: use whole homogenate, rather than nuclear pellet Compare the easy and rapid iodixanol method with the traditional sucrose method, in which a 1000 g pellet from the homogenate is suspended in 60% sucrose and layered over 65% sucrose.Compare the easy and rapid iodixanol method with the traditional sucrose method, in which a 1000 g pellet from the homogenate is suspended in 60% sucrose and layered over 65% sucrose.
13. Density of particles in iodixanol allows superior resolution The isolation of many widely-investigated organelles poses problems for sucrose gradients. All the major organelles of the light mitochondrial fraction possess seriously overlapping densities in sucrose gradients. In part this is due to the much higher osmolality of sucrose gradients compared to those of iodixanol (or Nycodenz) the organelles in sucrose gradients (in effect) approach a limiting density. It is for example necessary to lower the density of lysosomes artificially to resolve them in good yield from mitochondria. The isolation of many widely-investigated organelles poses problems for sucrose gradients. All the major organelles of the light mitochondrial fraction possess seriously overlapping densities in sucrose gradients. In part this is due to the much higher osmolality of sucrose gradients compared to those of iodixanol (or Nycodenz) the organelles in sucrose gradients (in effect) approach a limiting density. It is for example necessary to lower the density of lysosomes artificially to resolve them in good yield from mitochondria.
14. Purification of mitochondria (S12) An example of a simple discontinuous iodixanol flotation gradient for the isolation of mitochondria An example of a simple discontinuous iodixanol flotation gradient for the isolation of mitochondria
15. Isolation of peroxisomes I (S09) Light mitochondrial fraction layered on a 20-40% (w/v) iodixanol gradient
Centrifuged at 100,000g for 1h
Gradient unloaded dense end first Peroxisomes in particular benefit from the use of iodixanol (or Nycodenz) gradients their purity is significantly higher compared to isolates from sucrose or Percoll gradients Peroxisomes in particular benefit from the use of iodixanol (or Nycodenz) gradients their purity is significantly higher compared to isolates from sucrose or Percoll gradients
16. Isolation of peroxisomes II This simple linear iodixanol gradient, which can be executed in a fixed-angle rotor, resolves the peroxisomes from all the other major organelles in a light mitochondrial fraction. Only some residual endoplasmic reticulum (ER) can be detected. Yield and purity are both 90-95%. In Percoll the peroxisomes are much more seriously contaminated by ER.This simple linear iodixanol gradient, which can be executed in a fixed-angle rotor, resolves the peroxisomes from all the other major organelles in a light mitochondrial fraction. Only some residual endoplasmic reticulum (ER) can be detected. Yield and purity are both 90-95%. In Percoll the peroxisomes are much more seriously contaminated by ER.
17. LMF in self-generated gradient (S14) Sometimes the aim of the gradient is not to isolate a particular organelle at the highest purity but to achieve a distinctive separation of all the organelles so that the location of some other function or component can be assessed. The ability of iodixanol to form self-generated gradients (see Slides 10-18 of Training File 2) makes this a very easy task. In the example shown in this slide the light mitochondrial fraction is simply adjusted to a 17.5% iodixanol and centrifuged for 3 h in a suitable rotor. Sometimes the aim of the gradient is not to isolate a particular organelle at the highest purity but to achieve a distinctive separation of all the organelles so that the location of some other function or component can be assessed. The ability of iodixanol to form self-generated gradients (see Slides 10-18 of Training File 2) makes this a very easy task. In the example shown in this slide the light mitochondrial fraction is simply adjusted to a 17.5% iodixanol and centrifuged for 3 h in a suitable rotor.
18. Vesicle/cytosol separation (S36) The determination of whether a protein resides in the cytosol or is membrane-bound forms an important part of many subcellular membrane studies. A simple method is to add OptiPrep (or a dense Nycodenz solution) to a vesicle+cytosol sample to adjust it to approx 1.16 g/ml. Then to layer a 1.14 g/ml and 1.05 g/ml solutions on top. During the centrifugation the vesicles migrate to the top interface and the cytosolic proteins remain in, or start to sediment through, the sample zone. This is a much more efficient method than placing the sample on top of a density barrier.The determination of whether a protein resides in the cytosol or is membrane-bound forms an important part of many subcellular membrane studies. A simple method is to add OptiPrep (or a dense Nycodenz solution) to a vesicle+cytosol sample to adjust it to approx 1.16 g/ml. Then to layer a 1.14 g/ml and 1.05 g/ml solutions on top. During the centrifugation the vesicles migrate to the top interface and the cytosolic proteins remain in, or start to sediment through, the sample zone. This is a much more efficient method than placing the sample on top of a density barrier.
19. The plasma membrane contains many specialized sub-domains and one of these, the lipid raft, is commonly separated in an iodixanol gradientThe plasma membrane contains many specialized sub-domains and one of these, the lipid raft, is commonly separated in an iodixanol gradient
20. Isolation of detergent-insoluble membranes (S33) The simple standard methodology is to isolate rafts as detergent-insoluble (detergent-resistant) membranes. Triton X100 (or some other non-ionic detergent) is included in all the solutions and a post-nuclear supernatant is adjusted to approx. 40% iodixanol. Two lower concentration iodixanol solutions and a small volume of homogenization medium (HM) are layered on top and during the centrifugation the rafts float to the top interface. Sometimes the 20% OR 35% iodixanol layer is omitted. The reproducibility of the iodixanol gradient is better than that of the corresponding sucrose gradient.The simple standard methodology is to isolate rafts as detergent-insoluble (detergent-resistant) membranes. Triton X100 (or some other non-ionic detergent) is included in all the solutions and a post-nuclear supernatant is adjusted to approx. 40% iodixanol. Two lower concentration iodixanol solutions and a small volume of homogenization medium (HM) are layered on top and during the centrifugation the rafts float to the top interface. Sometimes the 20% OR 35% iodixanol layer is omitted. The reproducibility of the iodixanol gradient is better than that of the corresponding sucrose gradient.
