WO2000066723A1 - Method of ultrafiltration - Google Patents
Method of ultrafiltration Download PDFInfo
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- WO2000066723A1 WO2000066723A1 PCT/US2000/011926 US0011926W WO0066723A1 WO 2000066723 A1 WO2000066723 A1 WO 2000066723A1 US 0011926 W US0011926 W US 0011926W WO 0066723 A1 WO0066723 A1 WO 0066723A1
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- WIPO (PCT)
- Prior art keywords
- pressure differential
- membrane
- constant pressure
- ultrafiltration
- volume
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Classifications
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12N—MICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
- C12N15/00—Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
- C12N15/09—Recombinant DNA-technology
- C12N15/10—Processes for the isolation, preparation or purification of DNA or RNA
- C12N15/1003—Extracting or separating nucleic acids from biological samples, e.g. pure separation or isolation methods; Conditions, buffers or apparatuses therefor
- C12N15/1017—Extracting or separating nucleic acids from biological samples, e.g. pure separation or isolation methods; Conditions, buffers or apparatuses therefor by filtration, e.g. using filters, frits, membranes
Abstract
A process for ultrafiltration using constant pressure differential as the driving force is disclosed. This process is particularly suited for use in concentrating or purifying proteins and/or nucleic acids, often without any need for one or more diafiltration steps. The process is particularly suited for small volume applications, such as small concentrator devices and multiple well plates that typically use starting volumes of liquids of less than about 500 microliters. The steps include adding a liquid volume above an ultrafiltration membrane and applying a constant pressure differential at a force and length of time to achieve the desired concentration on the upstream side of the membrane. The concentrate is then diluted or removed for further processing.
Description
METHOD OF ULTRAFILTRATION Related Cases
This case is related to USSN 60/132,369, filed May 5, 1999,entιtled "Method of
Ultrafiltration, designating Jack T Leonard and Steve Toth as co-inventors
The present invention relates to a method of ultrafiltration More particularly, it relates to a method for ultrafiltration using constant pressure differential as the driving force
Background of the Invention
Methods for ultrafiltration have relied on centrifugal forces to force the liquid component through an ultrafiltration membrane Typically, positive pressure has been used when large volumes of fluid are to be filtered (e g stirred cells or spiral UF cartridges) Centrifugal force is the prevalent method used with small ultrafiltration devices, although some positive pressure attempts have been made with varying and impracticable results
Ultrafiltration with small devices is becoming the staple in biological research such as DNA and protein research as researchers look to use smaller and smaller quantities in their research and as automation becomes more accepted Such devices are either a single filter device such as is shown in US Patents 4,632,761 , 4,772,972 and 4,832,851 or multiple well plates as is known from US Patents 5,141 ,718 and 5,223,133
The process of ultrafiltration in such devices is used to fractionate different sized molecules from each other This may be used to remove impurities from the process used to develop or separate out the desired component or to separate the desired component from any other components in the liquid The process results in a concentration of a retained solute above the membrane with a low molecular weight component passing through the membrane thereby removing it from the fluid being filtered The liquid/ solid material retained above the membrane is called the retentate and the liquid below the membrane is called the filtrate
In order to the remove or reduce the concentration of impurities such as low molecular weight components and various salts in the retentate, the material must be diluted by the addition of a liquid While trying to affect a fractionation, low concentration factors sometimes delivered by
centrifugal ultrafiltration requires the use of multiple dilution and filtration steps (i e diafiltration) to deliver the retentate in a concentrated and sufficiently pure and relatively salt-free form This is particularly true for small volume devices because of the low head height associated with these small volumes which results in low driving pressures Moreover in the centrifugal process, the pressure doesn't remain constant Rather it is always and continuously decreasing during the process as the volume and thus the head height decreases during filtration in that the pressure is determined solely by the height of the liquid column above the membrane and the g-force applied to the membrane face However as the centrifuge process proceeds and the head height lessens, the pressure declines dramatically, resulting in flux decay (reduction in filtration rate and efficiency)
Additionally, acceptable designs for centrifugal ultrafiltration devices and filtrate retrieval components are constrained by the centrifuge rotor dimensions and the strength of the plastics These constraints, in turn, limit the maximum g-force that a given device can tolerate before failing Ultimately, the membrane type and active membrane area, strength of the plastic housing, g-force, and the ability to achieve and maintain adequate head height will determine the performance of the centrifugal ultrafiltration device
Vacuum manifolds are well accepted and widely used in many devices using microporous or macroporous filters Positive pressure manifolds have also been suggested for microporous applications However, ultrafiltration devices have not been designed to fit either manifold Moreover, there is a widely held belief in the art that ultrafiltration with vacuum is far too slow to be practical In fact, this perception is held even for larger ultrafiltration devices where initial volumes are high for a fixed surface area of ultrafiltration membranes This has led to the state of the art where centrifugal force is used to practice ultrafiltration of small samples
US Patent 5,679,310 suggests using a vacuum to filter a multiple well plate which utilizes ultrafiltration or microporous hollow fibers or other large surface area configurations of membranes instead of flat sheet membranes The hollow fibers are reported to be used in lieu of flat sheet membranes in order to increase the total surface area of the membrane over that available with a flat sheet To the knowledge of the inventors, this product has never been commercialized
The device has several drawbacks First, it uses a highly three dimensional filter (hollow fiber) to increase overall surface area, but then severly restricts the ability of the filter to discharge filtrate from the well through the use of one or more small openings which connect the hollow fiber
lumen to the exterior of the well The extremely small surface area available for filtration from the well as compared to a flat sheet (estimated as being less than about 20% of that of a flat sheet), results in a filtration rate that would not be close to that achieved with centπfugation on a flat sheet Perhaps this is why vacuum was suggested, as a means for increasing the rate to a level closer to that of a flat sheet with centπfugation Second, due to its 3-dιmensιonalιty, recovery of retentate from the well using conventional techniques such as pipetting is difficult, if not impossible Last and most importantly, as the level of fluid in the well decreases, the flux and available filtration area also dramatically decline as less and less filter area is below the fluid level and thus rendering it progressively less capable of filtering the remaining fluid leading to the same flux decay problems found with flat sheet devices using centπfugation
What is desired is a process which overcomes the problems of centπfugation in flat sheet ultrafiltration or vacuum in 3-D hollow fiber ultrafiltration especially in small volume single or multiple well devices and which provides such filtration in a time comparable or shorter than that achieved with the centnfugation process today The present invention provides such a process
Summary of the Invention
The present invention provides a process for ultrafiltration using a constant pressure differential as the driving force for the filtration process High flow rates can be maintained for durations sufficient for most applications using this process This allows for separation of low volumes of starting materials in a shorter period of time than can be achieved with centnfugation Additionally, constant pressure differential driven ultrafiltration is not subject to flux decay over time with non-polarizing solutes as occurs in centrifugal ultrafiltration The consequence of either process is that much higher concentration factors can be achieved using constant pressure differential driven ultrafiltration as compared to centrifugal ultrafiltration Additionally, although flux decay is observable using constant pressure differential driven ultrafiltration with polarizing solutes such as concentrated proteins, constant pressure differential driven ultrafiltration is faster than centrifugal ultrafiltration in most situations Lastly, the process of constant pressure differential driven ultrafiltration reduces or eliminates the need for time-consuming repeat dilutions and filiations that are frequently required with centnfugation to remove low molecular weight contaminants
The present process involves taking an ultrafiltration device containing one or more ultrafiltration wells, each well containing an ultrafiltration membrane and applying a constant pressure differential to the liquid within the device in order to cause a constant pressure differential driven ultrafiltration to occur The constant pressure differential is applied at a force and for a time sufficient to achieve a desired level of ultrafiltration
It is an object of the present invention to provide a process for ultrafiltration comprising the steps of providing a device containing an ultrafiltration membrane, said membrane having an upstream and downstream sides, said device having a first reservoir adjacent the upstream side of the membrane for holding a volume of liquid to be filtered and having a second reservoir or drain on the downstream side of the membrane for collecting liquid that is filtered from the sample through the membrane, placing a liquid volume into the first reservoir of the device, and applying a constant pressure differential force to the liquid at a force and time sufficient to cause substantially all of the liquid to pass from the first reservoir through the membrane to the second reservoir or drain It is another object of the present invention to provide a process for the concentration of nucleic acids and proteins comprising the steps of providing an ultrafiltration membrane having an upstream and a downstream side, said membrane having a molecular cutoff between 100 Daltons (0 I kDaltons(kD)) and 300kD, adding a volume of liquid containing a biological material selected from the group consisting of nucleic acids, proteins and blends thereof and subjecting the material to a constant pressure differential until a desired concentration of the biological material on the upstream side is reached
These and other objects of the present invention will become obvious from the specification and appended claims below
In The Drawings
Figure 1 shows a graph depicting the rate and overall time required to filter a given volume of sample by constant pressure differential and centnfugation (500 μl)
Figure 2 shows a graph depicting the rate and overall time required to filter a given volume of sample by constant pressure differential and centnfugation (300 μl) Figure 3 shows a close up of a portion of the graph of Figure 2
Figure 4 shows a graph depicting the rate and overall time required to filter a given volume of sample by constant pressure differential and centnfugation (1 OOμl)
Figure 5 shows a graph depicting the effect of increasing the constant pressure differential over that used in Figures 1-4 (40psι) Figure 6 shows a graph of the results from Example 1 utilizing a negative constant pressure differential
Figure 7 shows a graph with the results from Example 2 utilizing a positive constant pressure differential
Detailed Description of the Invention
The present invention is a process for the ultrafiltration and/or concentration of materials, preferably biological materials such as nucleic acids and/or proteins (although other materials typically filtered by ultrafiltration may be used) The process involves applying a constant pressure differential force to the material to be filtered for a period of time and at a force sufficient to cause the desired level of filtration or concentration
By " constant pressure differential " it is meant either a positive pressure or negative (or vacuum) pressure Unlike the pressure of the centrifugal method in which the pressure is always decreasing over time due to a reduction in head height of the liquid, in a constant pressure differential process the pressure acting on the liquid can remain constant over the filtration cycle Additionally, as the pressure is independent of head height of the liquid on which it is acting it may even be increased over time in order to drive the filtration process to completion It is also within this definition to have a decrease in pressure over time if desired, however unlike in centnfugation, this decrease is controlled and is independent of head height of the liquid thus reducing or eliminating flux decay
Ultrafiltration membranes are typically rated by their nominal molecular weight cutoff (le the largest sized molecule which can pass through the particular membrane) rather than by average pore size (as with microfiltration membranes) Typically, molecular cutoffs in the range of from about 100 Daltons (100D) to about 500 kiloDaltons (500kD) are the preferred membranes useful in the present device Preferably the range is from about 100D to about 300kD and more preferably
from about 3kD to about 300 kD Ultrafiltration membranes can be made from a variety of materials including but not limited to polyamides, polysulphones, polyethersulphones polyarylsulphones, polyphenylsulphones, cellulosics, regenerated celluloses and polyvinylidene fluoride They may be symmetrical or asymmetrical with asymmetrical designs being preferred One preferred method of the present invention is to use a small volume UF filtration device such as a single well device like Ultrafree® or Centπcon® or Microcon® single well device available from Mil pore Corporation, see U S Patent 4,632,761 These devices are designed for centrifugal filtration and are simply inserted into a centrifuge that is spun at certain revolutions to give a g-force sufficient to drive the ultrafiltration In the present method, a constant pressure differential force is applied to the liquid in the device and the constant pressure differential becomes the driving force for the filtration process rather than the traditional g-force of centnfugation When using a positive pressure differential (positive pressure), it is typically applied to the topside of the liquid to drive the liquid through the membrane When a negative pressure differential or vacuum is used, the pressure is typically applied to the downstream side of the membrane so as to act on the bottom of the liquid and draw it through the membrane
The same process can be used with a multiple welled plate, such as is disclosed in U S Patents 4,902,481 and 5,047,215 These plates are commercially available in a number of configurations, generally containing from about 6 to 1536 wells per plate The most common plate has 96 wells and is available from Millipore Corporation as the MultiScreen® 96 well plate In the process according to the present invention, the plate can be mounted on top of a vacuum manifold such that the vacuum is applied to the downstream side of the filter A sample to be filtered is placed into one or more of the wells and the vacuum is applied at a force and time sufficient to reach the desired level of filtration Alternatively a positive manifold can be mounted on the upstream side of the membrane and a positive pressure differential can be applied to the liquid at a force and time sufficient to achieve the desired filtration
The level of force (whether positive or negative) applied depends upon a number of factors among them are the amount of sample to be filtered, the type of membrane used (the molecular cutoff of the membrane, its strength and thickness), the active filtration area of the membrane, the speed at which the filtration is to occur and the level of polarization of the sample The strength of the plastic is a much lesser variable especially as compared to centrifugal devices where plastic strength of the device in large part controls the g-force that can be supplied
and therefore the rate and amount of filtration which can be achieved These means that thinner less robust devices may be used and achieve comparable or superior filtration rates and percentages One such advantage is the ability to use vacuum-formed trays especially with a vacuum driven or low positive pressure driven pressure differential process, something that is not available with centrifugal operated devices where such trays cannot withstand the required g-force for filtration to occur
Additionally, unlike centrifugal filtration, constant pressure differential filtration is completely independent of the ability to achieve and maintain a head height meaning that the process is not typically subject to any flux decay at non-polarizing concentrations of solute Typically, with small volumes, the consequence is that much higher concentration factors are achievable with constant pressure differential driven ultrafiltration as can be achieved with centnfugation within the same amount of time
Normally, the volumes of liquid in which this process can be used will vary, with a high value of about 2 milliliters More typically, it is used with volumes of less than 1 milliliter and preferably below 0 5 milliliters (500 microliters) This is clearly shown in the graph of Figure 1 As can be clearly seen there is an upper limit at which, due to sufficient head height, centnfugation is just as quick as the constant pressure differential process of the present invention ( the exact level is dependent among other things upon the fluid used and the level of constant pressure differential and centnfugation used) However, as will be explained below in conjunction with diafiltration, even when the rates are clearly faster for centnfugation, there are other compelling reasons for still using the process of the present invention rather than centnfugation as it eliminates or lessens the need for diafiltration
At lower volumes, it is clear however that use of the constant pressure differential of the present invention is clearly faster than that of centnfugation The point at which the constant pressure differential process is faster than centnfugation is hereinafter referred to as the
"breakthrough point" Figure 2 shows just such an example Here, the breakthrough point is at about the 7 minute mark As shown in Figure 2, when using a small volume, about 0 300 milliliters, the present process is about 60% faster than centnfugation
Figure 3 is a close up of the graph of Figure 2 for the last 0 020 milliliters of fluid to be filtered Here the differences between the present invention and centnfugation and the breakthrough point can be clearly and dramatically shown
Figure 4 shows the same effect with even smaller starting volumes of fluid Here, as shown, the present process is about 5 times faster that of centnfugation
Figure 5 shows the effect that varying the level of the constant pressure differential has on the process In this example, a 3 5 fold increase in the constant pressure differential over that applied in Figure 1 results in an almost 6 fold increase in filtration speed Additionally the breakthrough point occurs at about 1 minute as compared to 7 minutes for that of Figure 1
Flux decay may occur in filtering materials that have a high level of polarizing characteristics In those instances, some flux decay may be observed during filtration by the present process, but this is independent of head height and has to do with the inherent properties of the material being filtered This means that smaller starting quantities of sample may be used and high levels of ultrafiltration and recovery can be achieved at satisfactory rates even with the presence of such polarizing materials, something that is not always possible with centrifugal processes
The constant pressure differential may be negative, e g a reduced pressure( below atmospheric) or a vacuum or positive e g above atmospheric
Typically, a negative pressure differential or vacuum force of from about 5 inches Hg to about 27 inches Hg can be used (169-914 millibars) More preferably from about 10 to about 27 inches (338-914 millibars) can be used The level of vacuum force can be easily varied by the user to fit the desired parameters of the system, the rate of ultrafiltration desired and the sample he/she is using
Typically, a positive pressure differential of from about 5 to about 80 psi can be used Higher pressures may be used with devices that have the strength to withstand such pressures More preferably, from about 40 to about 60 psi can be used The level of positive pressure can be easily varied by the user to fit the desired parameters of the system, the rate of ultrafiltration desired and the sample he/she is using
The amount of starting fluid to be filtered can vary widely However this process has been found particularly useful with small volumes of liquid which cannot typically generate or maintain a suitable head height Such volumes are generally under about 1000 microliters, preferably less than about 500 microliters and may be as little as 1 microliter An additional advantage of the process of the present invention is that the need for diafiltration (reduction of salts or contaminants by repeated dilutions in ultrapure water or solvent
followed by centrifugal filtration to remove the solvated impurities and salts) can be reduced or eliminated making this process of particular benefit to the biological research area where such diafiltration steps are time consuming and if not complete, can skew the results obtained
It has been known that a single pass centnfugation process will not remove all salts and other impurities from a biological sample Therefore, the normal protocol is to dilute the retentate in ultrapure water or a solvent and re-centπfuge the material one or more times in order to draw out a sufficient volume of these impurities
It has been discovered that in normal centnfugation, as the volume of liquid above the membrane gets below a certain level, typically below 1 microliter volume, evaporation of the liquid is primarily phenomenon responsible for the removal of the liquid, not ultrafiltration This is due to the low head height that results in little if any pressure being applied to the remaining liquid and thereby little if any filtration occurring Because of this, any impurity is simply dehydrated onto the surface of the filter When a reconstituting liquid is added to the retentate these materials simply dissolve into the liquid and remain with the retentate This explains the need for several diafiltration steps
It has been discovered that in using the constant pressure differential process of the present invention filtration remains the dominant means for removing these impurities (as it is independent of head height in order to function), thereby causing the impurities to pass through the membrane and out of the retentate to a much greater level than can be achieved with centnfugation Essentially all impurities are removed with the current process in a single pass whereas often less than 90% of all impurities are removed with a single pass using the traditional centnfugation process This allows one to reduce or to eliminate the need for diafiltration steps after filtration and provides a purer product for further use
As mentioned above, this process is particularly useful when starting with small volumes as the process is quicker than centnfugation Additionally when the desire is to remove impurities from a biological sample, this process may be used with larger starting samples even though the filtration time may be longer than that for a centnfugation process as it will result in a purer retentate with fewer if no diafiltration steps The overall time savings (filtration and diafiltration) can justify the apparent increase in filtration time Alternatively, one may combine the efficiencies of both processes to process large volumes of biological samples with higher resultant purity One may simply centrifuge the initial
volume until about 20% or less of the original volume remains (or about at least 80% of the initial volume has been removed by centnfugation) Thereafter, one applies the constant pressure differential process of the present invention to remove remaining impurities from the sample In doing so, one can substantially reduce the time needed to conduct the ultrafiltration as well as reduce or eliminate the need for several diafiltration steps
Example 1
One hundred microliters of distilled water were placed in all wells of 96-well ultrafiltration plates with a nominal molecular weight cut-off of 30 kD The plate was placed on top of a collection plate and it was centπfuged at 2,000 x g in a swinging bucket rotor Plates were also placed on a vacuum manifold, and a vacuum applied at 24 inches of Hg (12 psi) and the time required to "go to dryness" was determined The amount of solution remaining in the plates was determined by weighing on a microbalance after processing for specific time intervals The average amount of solution remaining per well was plotted as a function of time
(Figure 6) This figure illustrates that higher concentration factors are achievable by vacuum under these conditions, and that the experimental values closely fit the predicted values
Example 2
Centπcon ® centrifugal ultrafiltration units with a nominal molecular weight cut-off of 30 kD were each loaded with 1 64 milliliters of distilled water The Centπcon® units were centπfuged at 2,000 x g in a swinging bucket rotor Another set of Centπcon® units were loaded with 1 64mιllιlιters of water and 40 psi of constant positive pressure was applied to the reservoir using compressed air The amount of solution remaining in the Centπcon® was determined by weighing on a microbalance after applying constant positive pressure, or after centnfuging for specific time intervals Retained liquid was recovered from the centπfuged Centπcon® units using the patented reverse spin technique
The average amount of solution remaining per Centπcon® unit was plotted as a function of time (Figure 7) Theoretical values, calculated using known flow rate for this membrane type, are also plotted This Figure illustrates that higher concentration factors are achievable by constant positive pressure under these conditions, and that the experimental values for both positive
pressure and centnfugation closely fit the predicted values Even after 17 minutes of centnfugation, 2 5 microliters on average could be recovered from the Centπcon® units by reverse spinning This provides evidence that centrifugal ultrafiltration is indeed asymptotic (/ e , does not achieve zero volume by active ultrafiltration)
What I Claim
Claims
Claims:
I ) A process for the concentration or purification of nucleic acids and proteins comprising the steps of providing an ultrafiltration membrane having an upstream and a downstream side, said membrane having a molecular cutoff between 100 D and 300kD, adding a volume of liquid of less than about 1000 microliters, said volume containing a biological material selected from the group consisting of nucleic acids, proteins and blends thereof and subjecting the volume to a constant pressure differential until a desired concentration of the biological material on the upstream side is reached. 2) A process for the concentration or purification of nucleic acids and proteins comprising the steps of providing an ultrafiltration membrane having an upstream and a downstream side, said membrane having a molecular cutoff between 100 D and 300kD, adding a volume of liquid containing a biological material selected from the group consisting of nucleic acids, proteins and blends thereof and subjecting the material to centnfugation until at least about 350 microliters or less of the initial volume remains, then subjecting the remaining volume to a constant pressure differential until a desired concentration of the biological material on the upstream side is reached. 3) The process of claim 1 wherein the constant pressure differential is a vacuum from about 169 millibars to about 914millibars 4) The process of claim 2 wherein the constant pressure differential is a vacuum from about 169 millibars to about 914millibars
5) The process of claim 1 wherein the constant pressure differential is a positive pressure from about 5 to about 80 psi.
6) The process of claim 2 wherein the constant pressure differential is a positive pressure from about 5 to about 80 psi.
7) The process of claim 1 wherein the device is a single well device.
8) The process of claim 1 wherein the device is a multiple well device.
9) The process of claim 1 wherein the device is a 96 well plate.
10) The process of claim 1 wherein the number of wells in the plate is from about 6 to about 1536.
I I) The process of claim 2 wherein the device is a single well device.
12) The process of claim 2 wherein the device is a multiple well device.
13) The process of claim 2 wherein the device is a 96 well plate.
14) The process of claim 2 wherein the number of wells in the plate is from about 6 to about 1536. 15) The process of claim 1 wherein the membrane has a molecular cutoff of from about
100 Daltons to about 500 kDaltons.
16) The process of claim 2 wherein the cutoff is from about 3 to about 300 kDaltons.
17) The process of claim 1 wherein the membrane is made of a material selected from the group consisting of polyamides, polysulphones, polyethersulphones polyarylsulphones, cellulosics, regenerated celluloses, polyolefins such as polyethylene and polypropylene and polyvinylidene fluoride.
18) The process of claim 2 wherein the membrane is made of a material selected from the group consisting of polyamides, polysulphones, polyethersulphones polyarylsulphones, cellulosics, regenerated celluloses, polyolefins such as polyethylene and polypropylene and polyvinylidene fluoride.
19) The process of claim 1 wherein the starting volume of liquid is less than about 500 microliters.
20) The process of claim 1 wherein the starting volume of liquid is less than 350 microliters. 21) The process of claim 1 wherein the process is free of a diafiltration step.
22) The process of claim 2 wherein the process is free of a diafiltration step.
Priority Applications (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| EP00928724A EP1144619A1 (en) | 1999-05-04 | 2000-05-02 | Method of ultrafiltration |
| DE1144619T DE1144619T1 (en) | 1999-05-04 | 2000-05-02 | METHOD FOR ULTRAFILTRATION |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US60/132,369 | 1999-05-04 | ||
| US18235700P | 2000-02-14 | 2000-02-14 | |
| US60/182,357 | 2000-02-14 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| WO2000066723A1 true WO2000066723A1 (en) | 2000-11-09 |
Family
ID=22668106
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| PCT/US2000/011926 WO2000066723A1 (en) | 1999-05-04 | 2000-05-02 | Method of ultrafiltration |
Country Status (1)
| Country | Link |
|---|---|
| WO (1) | WO2000066723A1 (en) |
Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2001079486A2 (en) * | 2000-04-13 | 2001-10-25 | Millipore Corporation | Method and apparatus for plasmid recovery involving ultrafiltration |
| WO2001094574A2 (en) * | 2000-06-07 | 2001-12-13 | Amersham Biosciences Corp | Method and apparatus for purifying nucleic acids |
| GB2375764A (en) * | 2001-01-19 | 2002-11-27 | Millipore Corp | Improved recovery of linear nucleic acids by salt dilution and/or reduced pressure prior to continuous pressure differential ultrafiltration |
| US6498240B1 (en) | 1999-09-17 | 2002-12-24 | Millipore Corporation | Method for sequencing reaction cleanup by constant pressure diffential ultrafiltration |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4690754A (en) * | 1985-03-12 | 1987-09-01 | Toyo Soda Manufacturing Co., Ltd. | Filter device for a minute volume of liquid |
| WO1987007645A1 (en) * | 1986-06-04 | 1987-12-17 | The London Hospital Medical College | A method of sequencing nucleic acids |
| EP0431905A1 (en) * | 1989-12-06 | 1991-06-12 | Tosoh Corporation | Method for purifying phage DNA |
| WO1992013963A1 (en) * | 1991-01-30 | 1992-08-20 | Hyman Edward D | Method for preparation of closed circular dna |
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2000
- 2000-05-02 WO PCT/US2000/011926 patent/WO2000066723A1/en not_active Application Discontinuation
Patent Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4690754A (en) * | 1985-03-12 | 1987-09-01 | Toyo Soda Manufacturing Co., Ltd. | Filter device for a minute volume of liquid |
| WO1987007645A1 (en) * | 1986-06-04 | 1987-12-17 | The London Hospital Medical College | A method of sequencing nucleic acids |
| EP0431905A1 (en) * | 1989-12-06 | 1991-06-12 | Tosoh Corporation | Method for purifying phage DNA |
| WO1992013963A1 (en) * | 1991-01-30 | 1992-08-20 | Hyman Edward D | Method for preparation of closed circular dna |
Non-Patent Citations (1)
| Title |
|---|
| M.C. LINHARES AND P.T. KISSINGER: "Capillary ultrafiltration : in vivo sampling probes for small molecules", ANAL. CHEM., vol. 64, 1992, pages 2831 - 2835, XP000938635 * |
Cited By (11)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US6498240B1 (en) | 1999-09-17 | 2002-12-24 | Millipore Corporation | Method for sequencing reaction cleanup by constant pressure diffential ultrafiltration |
| US6645722B2 (en) | 1999-09-17 | 2003-11-11 | Millipore Corporation | Method for sequencing reaction cleanup by constant differential pressure ultrafiltration |
| WO2001079486A2 (en) * | 2000-04-13 | 2001-10-25 | Millipore Corporation | Method and apparatus for plasmid recovery involving ultrafiltration |
| WO2001079486A3 (en) * | 2000-04-13 | 2002-06-13 | Millipore Corp | Method and apparatus for plasmid recovery involving ultrafiltration |
| US6759233B2 (en) | 2000-04-13 | 2004-07-06 | Millipore Corporation | Method of plasmid recovery and apparatus for doing so |
| US7297534B2 (en) * | 2000-04-13 | 2007-11-20 | Millipore Corporation | Method of plasmid recovery and apparatus for doing so |
| WO2001094574A2 (en) * | 2000-06-07 | 2001-12-13 | Amersham Biosciences Corp | Method and apparatus for purifying nucleic acids |
| WO2001094574A3 (en) * | 2000-06-07 | 2002-06-20 | Amersham Biosciences Corp | Method and apparatus for purifying nucleic acids |
| GB2375764A (en) * | 2001-01-19 | 2002-11-27 | Millipore Corp | Improved recovery of linear nucleic acids by salt dilution and/or reduced pressure prior to continuous pressure differential ultrafiltration |
| GB2375764B (en) * | 2001-01-19 | 2005-06-08 | Millipore Corp | Improved recovery of linear nucleic acids by salt dilution and/or reduced pressure prior to continuous pressure differential ultrafiltration |
| US7074333B2 (en) | 2001-01-19 | 2006-07-11 | Millipore Corporation | Recovery of linear nucleic acids by salt dilution and/or reduced pressure prior to continuous pressure differential ultrafiltration |
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