Patent Grant
9005417
Embodiments of the invention relate generally to microfluidic devices, and more specifically to methods and systems for performing microscale isoelectric fractionation.
Biological diagnostic techniques frequently require a purification process be performed on a sample prior to analysis. An unprocessed serum sample may contain as many as 105-106 different protein species at various concentrations. In proteomic diagnostics, accordingly, analytes of interest in a serum sample may be obscured by other protein species in the sample. Accordingly, microfluidic assay techniques typically require an off-chip purification technique such as dialysis, centrifugation, or desalting, prior to analysis. Requiring an off-chip purification step may limit the usefulness of microfluidic analysis techniques. Without the ability to receive and analyze a raw sample, the microfluidic device may not also serve as the collection point for a raw sample. Rather, the raw sample may first be processed in a macroscale device and later introduced into the microfluidic device for analysis.
Isoelectric fractionation is a technique for electrokinetically separating analytes in solution based on their isoelectric point. The isoelectric point of an analyte is the pH at which the analyte acquires no net charge. For example, proteins are composed of a variety of amino acid groups which act together to give the protein its overall charge. At the isoelectric point of the protein, the exchange of protons with the solution (protonation and deprotonation) will be balanced, and the protein acquires no net charge. At a pH below the isoelectric point of the protein, protonation typically dominates and the protein acquires a net positive charge. At a pH above the isoelectric point of the protein, deprotonation dominates and the protein acquires a net negative charge.
The tube 100 is typically around a half-inch in diameter, and several inches long. The tube 100 includes individual compartments 105, 110, 115, and 120. Each chamber may be connected to the next by, for example, threaded connectors. Each compartment is separated from the next by a membrane cartridge 106, 111, 116, and 121, respectively. Each membrane cartridge 106, 111, 116, and 121 contains a porous membrane having a constant and specific pH value. The membrane cartridges and compartments may have O-rings or other sealing devices separating the individual compartments. The pH values of the membranes increase from a first end 130 of the tube 100 to a second end 135 of the tube 100. A sample in solution is loaded into the tube at any point and is separated using electrophoretic transport.
Electrophoretic transport involves applying an electric field across the tube 100. Accordingly, an electric field 140 is generated by applying a voltage across an anode 145 at the first end 130 of the tube and a cathode 150 at the second end 135 of the tube 100. Positively charged analytes will be transported through the tube 100 in the direction of the electric field 140, toward the cathode 150, and negatively charged analytes in the opposite direction. The analytes will pass through the membrane cartridges 106, 111, 116, 121 until they reach the compartment corresponding to their isoelectric point, at which point they will have no net charge, and will no longer move through the tube 100 by electrophoresis. In this manner, the analytes may be separated according to their isoelectric point. Following fractionation, the isolated samples in the compartments 105, 110, 115, and 120 may be removed for further analysis.
Macroscale isoelectric fractionation, as described above and with reference to
Certain details are set forth below to provide a sufficient understanding of embodiments of the invention. However, it will be clear to one skilled in the art that embodiments of the invention may be practiced without various of these particular details. In some instances, well-known materials, chemical components, buffers or other additives, analytes, electrical components, material processing and fabrication techniques, have not been shown in detail in order to avoid unnecessarily obscuring the described embodiments of the invention.
Embodiments of the present invention provide devices and methods for performing microscale isoelectric fractionation (AF). Devices according to embodiments of the present invention generally include a channel having a dimension of around 1 mm or less. In some embodiments, 500 μm or less. In some embodiments, the devices have a dimension of around 100 μm or less. Other dimensions may be used, as generally described below.
Two membranes 210, 215 are positioned in the microchannel 205. As will be described further below, the membranes each have a different pH, making the microchannel structure 200 suitable for performing isoelectric fractionation. General features of the microchannel structure 200 having been described, a discussion of embodiments for making the microchannel structure 200, including the membranes 210, 215 will now be discussed with reference to
The channel 205 itself may be formed by generally any material suitable for forming a channel of the dimensions described above and for containing the membranes which will be further described. Glass, including fused silica, may be used to form the channel 205 in some embodiments. In the embodiments shown in
Accordingly, a bottom surface and sidewalls of the microchannel 205 may be defined by the glass substrate 301. A top surface of the microchannel 205 may be defined by a material integral to the substrate 301 or adhered or bonded to the substrate 301, such as an upper substrate 302. The upper substrate 302 may also be glass, fused silica, PDMS, PMMA, cyclic olefin copolymer, polycarbonate, or other material compatible with the techniques and processes described herein. At least one surface of the channel 205 may be formed of a transparent material for ease in exposing all or portions of the channel 205 to a light source, as will be further described below.
After forming the microchannel 205, the surfaces of the microchannel 205 may be treated to promote adhesion to the membranes 210, 215. In some embodiments, the membranes 210, 215 are polyacrylamide membranes and a surface treatment prior to the formation of the membranes may include coating one or more of the interior surfaces of the microchannel 205 with an acrylate-terminated self-assembled monolayer using a process of incubation, rinsing, and drying. In one embodiment, the surface treatment includes conditioning the microchannel 205 with 1M aqueous NaOH, rinsing with deionized water, and vacuum drying the microchannel 205. Introduction of fluids into the microchannel 205 may occur through any known methods, including by pressure-driven flow. A 2:3:5 (volume ratio) mixture of 3-(trimethoxysilyl)propyl methacrylate, glacial acetic acid, and deionized water that has been sonicated and degassed, is then loaded into the microchannel 205. The microchannel 205 is incubated for about 30 minutes, rinsed with a 3:7 (v/v) mixture of acetic acid and water, rinsed with deionized water, and dried with a vacuum. This process leaves an acrylate terminated self-assembled monolayer 305 on the surfaces of the microchannel 205. The self-assembled monolayer 305 is shown in
The membranes 210, 215, according to embodiments of the present invention are regions of polyacrylamide gels. Generally, the gels are formed by introducing an aqueous solution including acrylamide monomer, bisacrylamide crosslinker, and a photoinitiator into the microchannel 205. The membranes 210, 215 may then be formed by polymerizing the solution by exposing the desired membrane area to a UV light source. The pH of the gel may be controlled by introducing calculated amounts of acrylamido buffers (such as IMMOBILINE®) into the aqueous acrylamide monomer solution. Various embodiments of suitable aqueous solutions and methods for polymerizing acrylamide gel regions are described in co-pending application Ser. No. 12/182,755 filed Jun. 30, 2008, entitled “Methods for providing and using solution gradients in microchannels,” and naming inventors Anson V. Hatch, Gregory J. Sommer, Amy E. Hen, and Anup K. Singh, the entire contents of which are hereby incorporated by reference for any purpose. The table below describes embodiments of suitable solutions at various pH levels. The quantity of acrylamide and the cross-linker bisacrylamide are listed as a total concentration percentage (T) and a concentration of the crosslinker (C), which can be calculated using the following equations:
The pH levels recited are by way of example only, and generally any pH level may be achieved by adjusting the recipe accordingly.
In one embodiment, the membranes 210, 215 are formed by flowing acrylamide monomer solutions of different pH through side channels (not shown) flanking the microchannel 205. This is illustrated schematically in
The microchannel 205 containing the acrylamide solution pH gradient 317 may then be exposed to a UV light source 319 through a mask 320. The regions of the solution exposed to the UV light source 319 are polymerized and form the membranes 210 and 215. By selecting the pH of acrylamide solutions A 310 and B 315, and the position along the microchannel 205 for UV light exposure, the pH of the membranes 210 and 215 can be selected. The pH of membrane 210 may be 6.0 while the pH of the membrane 215 may be 5.0 in the example of
Following polymerization, unpolymerized solution may be flushed out of the microchannel 205. Solution may be removed from the inlet and outlet of the microchannel 205, through side channels, such as the channels 220 and 230 in
Embodiments of methods for forming discrete membranes of different pH using an acrylamide solution pH gradient 317 and resultant devices are described in co-pending application Ser. No. 12/182,755 filed Jun. 30, 2008, entitled “Methods for providing and using solution gradients in microchannels,” and naming inventors Anson V. Hatch, Gregory J. Sommer, Amy E. Herr, and Anup K. Singh, the entire contents of which are hereby incorporated by reference for any purpose.
Accordingly, a process described above with reference to
The microchannel 205 and self-assembled monolayer 305 are formed as described above with reference to
The first acrylamide solution 410 having a pH of 5.0 is then flushed out of the microchannel 205 through the inlet, outlet, or side channel such as the side channels 220 and 230 in
As in the process described above with regard to
Although the methods described above result in the formation of two membranes 210 and 215, embodiments of the present invention may be employed to form any number of membranes in a microchannel, including 1, 2, 3, 4, 5, 6, 7, 8, 9, and 10 membranes. Some embodiments may have up to 20 membranes in a microchannel. Still more membranes may be formed in the channel in accordance with the length of the channel and the desired application, up to 100 membranes or even more. A well-controlled gradient may be generated up to centimeters long and membranes may be fabricated as close as about 100 microns apart. The membranes 210 and 215 described above have pH values—5.0 and 6.0 —that are 1 pH unit apart. However, embodiments of the present invention may be used to form membranes in a microchannel having pH values that are closer together or further apart, with the closest spacing being about 0.01 pH unit. To achieve the smaller resolutions, membranes may be formed by generating a shallow gradient by diffusion and then photopolymerizing membranes at different points along the gradient. Accordingly, the membrane 210 may have a pH of 5.0, for example, while the membrane 215 has a pH of 5.1. Accordingly, membranes may be provided having substantially any pH resolution from about 0.1 pH unit on up. As will be described further below, the selection of pH of the membranes will affect the resolution of the isoelectric fractionation that may be performed in the microchannel 205.
After formation of the membranes 210, 215 through using embodiments of the methods described above, the microchannel 205 may be filled with an aqueous solution of acrylamide monomer at neutral pH and the entire microchannel 205 exposed to the UV light source 319 to photopolymerize an acrylamide gel throughout the microchannel 205. The microchannel 205 would then contain a continuous gel with regions of specific pH at the membranes 210, 215. In other embodiments, the microchannel 205 is not filled with acrylamide gel, and an aqueous or other fluid medium may fill the channel, including the region between the membranes 210 and 215.
The membranes 210, 215 generally block fluid flow in the microchannel 205; however, the membranes 210, 215, formed of polymerized acrylamide solution, are sufficiently porous to allow analytes to pass through the membrane. The microchannel structure 200 shown in
A sample is introduced to the microchannel 205, at the first end 250, or any location along the microchannel 205, or any combination of microchannel locations. The sample may generally be any fluid containing target analytes for separation by the isoelectric fractionation techniques described below. Samples accordingly may include serum, urine, saliva, or other biological fluid samples. Analytes that may be separated according to the techniques described below include proteins, peptides, or other species in the sample that may be separated according to their isoelectric point.
The sample may be introduced into the microchannel 205 through any mechanism, including pressure driven flow. The sample may be stored in a sample reservoir in fluid communication with the microchannel 205. The sample reservoir may be integral with or separable from the microchannel structure 200. Analytes are then drawn into the microchannel 205, toward the membranes 210 and 215 using electrophoresis. An electric field 260 is generated in the microchannel 205 by applying a voltage between two electrodes 265, 270. Any suitable voltage generator and electrodes may be used to generate the electric field 260, and the electrodes 265, 270 may be integral to the microchannel structure 200, or they may be separate from the structure 200 and placed in sufficient proximity to the structure 200 to generate the electric field 260 in the microchannel 205. The particular voltage used will depend on the spacing of the electrodes 265, 270 and the analytes to be transported. In one embodiment, an electric field 260 of 330 V/cm may be sufficient to transport analytes through the microchannel 205.
Three analytes 275, 280, and 285 having different pH values are shown in
Under the influence of the electric field 260, the analytes 285, 280, and 275 are drawn from the first end 250 of the microchannel 205 toward the second end 290 of the microchannel. In higher pH environments, proteins are more negatively charged; accordingly, the proteins will be drawn toward the more positive electrode until they reach their isoelectric point at which they carry substantially no net charge. For example, the analyte 275 will not traverse through the membrane 210. Recall the membrane 210 has a pH of 6.0 and the analyte 275 has an isoelectric point of greater than 6.0. Accordingly, the analyte 275 will remain in the area of the microchannel 205 between the first end 250 and the membrane 210. The analytes 280 and 285, however, have isoelectric points less than 6.0, and will be drawn through the membrane 210 as shown, and toward the second membrane 215. The analyte 280, having an isoelectric point greater than 5.0, will not traverse through the second membrane 215 which has a pH of 5.0. Accordingly, the analyte 280 will remain in the region of the microchannel 205 between the first membrane 210 and the second membrane 215. The analyte 285, having an isoelectric point less than 5.0 will be drawn through the membrane 215, and will proceed toward the second end of the microchannel 290. The analyte 285 may be transported out of the microchannel 205 and into a waste or other reservoir in fluid communication with an outlet of the microchannel 205
During the fractionation process, one or more E-fields generally perpendicular to the fractionation channel may also be applied to help retain analytes within the fractionation channel. This would reduce loss occurring at any cross-channel intersections by, for example, diffusion outside of the centrally applied field.
The microscale isoelectric fractionation techniques described may also enable preconcentration of analytes. The local concentration of an analyte within each pH range may be increased with continued fractionation. The concentrated analyte may then be used in any analytic or other technique.
In this manner, analytes having an isoelectric point over 6.0 will be collected in the region between an inlet of the microchannel 205 and the membrane 210. Analytes having an isoelectric point between 6.0 and 5.0 will be collected in the region between the membranes 205 and 210. Analytes having an isoelectric point less than 5.0 will be collected in a region following the membrane 215, or in a waste reservoir. Although three regions of separation are achieved in the embodiment of
Once fractionated, analytes in the various regions may be transported to other locations. For example, the analyte 275 may be transported through an analyte collection microchannel 295. Transport through the analyte collection microchannel 295 may be achieved by, for example, applying an electric field (not shown) along the analyte collection microchannel sufficient to transport the analyte 275 by electrophoresis. In a similar manner, the analyte 280 may be transported through the analyte collection microchannel 297 by applying an electric field along the analyte collection microchannel sufficient to transport the analyte 280 along the analyte collection microchannel. The analyte collection microchannels may be placed at any location in fluid communication with the fractionation microchannel 205 containing the separated analytes. As shown in
As described above, microscale isoelectric fractionation may separate analytes on-chip through selected electrophoretic migration of the analytes through pH-specific polyacrylamide membranes. The membranes restrict molecules having isoelectric points below the pH of the membrane. By designing microfluidic channels having a serial array of membranes at various pH values, analytes may be separated and isolated into corresponding pH ranges. While macroscale isoelectric fractionation may take several hours to fractionate, microscale isoelectric fractionation may take only minutes due to the reduced length scales used.
Embodiments of devices and methods conducting micro scale isoelectric fractionation in a fractionation channel have been described above. Analytes may be separated according to their isoelectric point, allowing for pre-treatment of a sample containing a wide variety of analytes, such as serum or urine. Once fractionated, analytes of a particular pH range may be transported from the fractionation channel 205 for use in other analytic techniques. Since the fractionation occurred in a microfluidic device, the analytes of interest may be transported to analysis modules on the same chip, which may save time and cost.
The preparation module 525 is used to separate one or more analytes of interest from other species in a sample. Accordingly, microscale isoelectric fractionation is performed in the preparation module 525 according to methods described above. The microchannel structure 200 of
Analytes having a certain isoelectric point range may then be moved into the transport module through analyte collection microchannels 540, 295, 297, 545, and 550. Transport may occur through any means, including pressure or pump driven flow, or electrophoresis. The transport module 535 includes transport channel 555. So, for example, analytes having an isoelectric point of between 5.0 and 6.0 may be fractionated into the region between the membranes 210 and 215 as described above. Those analytes may then be transported into the transport channel 555 for analysis. Although only one assay module 530 is shown in
Turning now to the assay module 530, analytes from the transport channel 555 are introduced into the assay module 530 and may be mixed with reagents introduced at reagent introduction channels 560, 562, 564. The specific reagents used will depend on the analyte and the assay technique performed by the assay module 530. In the embodiment shown in
Other microfluidic components may be integrated into the microfluidic system of
As described above, sample may be introduced at an inlet 520, fractionated in the preparation module 525 to group analytes in the sample according to isoelectric point. Only analytes having a certain range of isoelectric points may then be transported in the transport module 535 to the assay module 530 for analysis. In this manner, a sample may be prepared on a microfluidic chip for later analysis on the same chip or within the same microfluidic system. Off-chip sample preparation processes may be reduced or eliminated.
From the foregoing it will be appreciated that, although specific embodiments of the invention have been described herein for purposes of illustration, various modifications may be made without deviating from the spirit and scope of the invention.
The United States Government has a paid-up license in this invention and the right in limited circumstances to require the patent owner to license others on reasonable terms as provided for by the terms of contract No. DE-AC04-94AL85000 awarded by the U.S. Department of Energy to Sandia Corporation.
| Number | Name | Date | Kind |
|---|---|---|---|
| 3376083 | Everhardus | Apr 1968 | A |
| 3844341 | Bimshas et al. | Oct 1974 | A |
| 4125375 | Hunter | Nov 1978 | A |
| 4156570 | Wardlaw | May 1979 | A |
| 4164690 | Muller et al. | Aug 1979 | A |
| 4282464 | Uzuka | Aug 1981 | A |
| 4380355 | Beardmore | Apr 1983 | A |
| 4554071 | Ruijten et al. | Nov 1985 | A |
| 4683579 | Wardlaw | Jul 1987 | A |
| 5000254 | Williams | Mar 1991 | A |
| 5197858 | Cheng | Mar 1993 | A |
| 5279936 | Vorpahl | Jan 1994 | A |
| 5296775 | Cronin et al. | Mar 1994 | A |
| 5297623 | Ogushi et al. | Mar 1994 | A |
| 5335143 | Maling, Jr. et al. | Aug 1994 | A |
| 5583746 | Wang | Dec 1996 | A |
| 5616974 | Yamada | Apr 1997 | A |
| 5635362 | Levine et al. | Jun 1997 | A |
| 5727928 | Brown | Mar 1998 | A |
| 5736787 | Larimer | Apr 1998 | A |
| 5794687 | Webster et al. | Aug 1998 | A |
| 5957659 | Amou et al. | Sep 1999 | A |
| 5963887 | Giorgio | Oct 1999 | A |
| 5979541 | Saito | Nov 1999 | A |
| 6050326 | Evans et al. | Apr 2000 | A |
| 6078468 | Fiske | Jun 2000 | A |
| 6153579 | Kim et al. | Nov 2000 | A |
| 6175495 | Batchelder | Jan 2001 | B1 |
| 6194798 | Lopatinsky | Feb 2001 | B1 |
| 6249071 | Lopatinsky et al. | Jun 2001 | B1 |
| 6319469 | Mian et al. | Nov 2001 | B1 |
| 6356435 | Davis et al. | Mar 2002 | B1 |
| 6379974 | Parce et al. | Apr 2002 | B1 |
| 6392720 | Kim | May 2002 | B1 |
| 6457955 | Cheng | Oct 2002 | B1 |
| 6525938 | Chen | Feb 2003 | B1 |
| 6545438 | Mays, II | Apr 2003 | B1 |
| 6619385 | Watanabe et al. | Sep 2003 | B2 |
| 6623860 | Hu et al. | Sep 2003 | B2 |
| 6638408 | Speicher et al. | Oct 2003 | B1 |
| 6659169 | Lopatinsky et al. | Dec 2003 | B1 |
| 6664673 | Lopatinsky et al. | Dec 2003 | B2 |
| 6685809 | Jacobson et al. | Feb 2004 | B1 |
| 6860323 | Cheng | Mar 2005 | B2 |
| 6873069 | Odagiri et al. | Mar 2005 | B1 |
| 6876550 | Sri-Jayantha et al. | Apr 2005 | B2 |
| 6879120 | Xi | Apr 2005 | B2 |
| 6955215 | Al-Garni et al. | Oct 2005 | B2 |
| 6960449 | Wang et al. | Nov 2005 | B2 |
| 6966357 | Herbert | Nov 2005 | B1 |
| 7021894 | Lopatinsky et al. | Apr 2006 | B2 |
| 7033747 | Gordon et al. | Apr 2006 | B2 |
| 7035102 | Holmes | Apr 2006 | B2 |
| 7044202 | Lopatinsky et al. | May 2006 | B2 |
| 7055581 | Roy | Jun 2006 | B1 |
| 7071587 | Lopatinsky et al. | Jul 2006 | B2 |
| 7100677 | Lee et al. | Sep 2006 | B2 |
| 7134839 | Horng et al. | Nov 2006 | B2 |
| 7136285 | Herbert | Nov 2006 | B1 |
| 7157049 | Valencia et al. | Jan 2007 | B2 |
| 7165413 | Symons | Jan 2007 | B2 |
| 7165938 | Lee et al. | Jan 2007 | B2 |
| 7265975 | Tsai | Sep 2007 | B2 |
| 7267526 | Hsu et al. | Sep 2007 | B2 |
| 7273091 | Bahl et al. | Sep 2007 | B2 |
| 7284596 | Larson | Oct 2007 | B2 |
| 7301771 | Hata et al. | Nov 2007 | B2 |
| 7304845 | Xia | Dec 2007 | B2 |
| 7312085 | Chou et al. | Dec 2007 | B2 |
| 7324339 | Foster Sr. | Jan 2008 | B2 |
| 7349212 | Xia et al. | Mar 2008 | B2 |
| 7381027 | Kaneko et al. | Jun 2008 | B2 |
| 7452507 | Renzi et al. | Nov 2008 | B2 |
| 7455501 | Horng et al. | Nov 2008 | B2 |
| 7458413 | Mok | Dec 2008 | B2 |
| 7481263 | Breier et al. | Jan 2009 | B2 |
| 7520314 | Hwang et al. | Apr 2009 | B2 |
| 7543457 | Crocker et al. | Jun 2009 | B2 |
| 7667969 | Khanna et al. | Feb 2010 | B2 |
| 7670102 | Chang et al. | Mar 2010 | B2 |
| 7695256 | Horng et al. | Apr 2010 | B2 |
| 7758810 | Lee et al. | Jul 2010 | B2 |
| 7836939 | Zimmerman et al. | Nov 2010 | B2 |
| 7896611 | Khanna et al. | Mar 2011 | B2 |
| 7900690 | Hawwa et al. | Mar 2011 | B2 |
| 7905712 | Huang | Mar 2011 | B2 |
| 7911791 | Refai-Ahmed et al. | Mar 2011 | B2 |
| 8337775 | Pugia et al. | Dec 2012 | B2 |
| 20010055812 | Mian et al. | Dec 2001 | A1 |
| 20020090307 | Cheng | Jul 2002 | A1 |
| 20020098535 | Wang et al. | Jul 2002 | A1 |
| 20020153251 | Sassi et al. | Oct 2002 | A1 |
| 20020164659 | Rao et al. | Nov 2002 | A1 |
| 20020170825 | Lee et al. | Nov 2002 | A1 |
| 20030013203 | Jedrzejewski et al. | Jan 2003 | A1 |
| 20030124719 | Woodside | Jul 2003 | A1 |
| 20030203504 | Hefti | Oct 2003 | A1 |
| 20030221963 | Bjellqvist et al. | Dec 2003 | A1 |
| 20040035556 | Jean | Feb 2004 | A1 |
| 20040072278 | Chou et al. | Apr 2004 | A1 |
| 20040109291 | Kannmacher et al. | Jun 2004 | A1 |
| 20040114327 | Sri-Jayantha et al. | Jun 2004 | A1 |
| 20040119354 | Takada et al. | Jun 2004 | A1 |
| 20040129567 | Auton et al. | Jul 2004 | A1 |
| 20050002163 | Lopatinsky | Jan 2005 | A1 |
| 20050087445 | Speicher et al. | Apr 2005 | A1 |
| 20050195573 | Huang | Sep 2005 | A1 |
| 20050274490 | Larson | Dec 2005 | A1 |
| 20060007656 | Symons | Jan 2006 | A1 |
| 20060021735 | Lopatinsky | Feb 2006 | A1 |
| 20060171654 | Hawkins et al. | Aug 2006 | A1 |
| 20060191792 | Herr et al. | Aug 2006 | A1 |
| 20070000268 | Crocker et al. | Jan 2007 | A1 |
| 20070041158 | Hornung | Feb 2007 | A1 |
| 20070231419 | Pelcz et al. | Oct 2007 | A1 |
| 20080069706 | Huang | Mar 2008 | A1 |
| 20080149484 | Tolley et al. | Jun 2008 | A1 |
| 20090145584 | Walsh et al. | Jun 2009 | A1 |
| 20090166004 | Lai et al. | Jul 2009 | A1 |
| 20100068754 | Kirakossian | Mar 2010 | A1 |
| 20100177480 | Koplow | Jul 2010 | A1 |
| 20100328887 | Refai-Ahmed et al. | Dec 2010 | A1 |
| 20110103011 | Koplow | May 2011 | A1 |
| Number | Date | Country |
|---|---|---|
| 0407169887 | Jul 1995 | JP |
| 2000-054978 | Feb 2000 | JP |
| 2000054978 | Feb 2000 | JP |
| 0200341902 | Dec 2000 | JP |
| 2006-037918 | Feb 2006 | JP |
| WO 0168225 | Sep 2001 | WO |
| WO2001068225 | Sep 2001 | WO |
| WO2010016963 | Oct 2010 | WO |
| Entry |
|---|
| Cui et al. Anal.Chem, 2005, 77, 7878-7886. |
| Long et al. Integration of nanoporous membranes for sample filtration/preconcentration in microchip electrophoresis Electrophoresis, 2006, 27,4927-4934. |
| Gusev et al., Capillary columns with in situ formed porous monolithic packing for micro high-performance liquid chromatography and capillary electrochromatography, J. Chromatogr. A, 1999, 273-290. |
| D. Ogle; A. Ho; T. Gibson; D. Rylatt; E. Shave; P. Lim; G. Vigh; “Preparative-scale isoelectric trapping separations using a modified Gradiflow unit”, Journal of Chromatography A, 2002, vol. 979, pp. 155-161. |
| G. V. Zilberstein; E. M. Baskin; S. Bukshpan; “Parallel pocessing in the isoelectric focusing chip”, Electrophoresis, 2003, vol. 24, pp. 3735-3744. |
| G. V. Zilberstein; L. E. Korol; S. Bukshpan; E. M. Baskin; “Parallel isoelectric focusing chip”, Proteomics, 2004, vol. 4, pp. 2533-2540. |
| G. V. Zilberstein; E. M. Baskin; S. Bukshpan; L. E. Korol; “Parallel isoelectric focusing II”, Electrophoresis, 2004, vol. 25, pp. 3643-3651. |
| D. Fologea; M. Gershow; B. Ledden; D. S. McNabb; J. A. Golovchenko; J. Li; “Detecting Single Stranded DNA with a Solid State Nanopore”, Nano Letters, 2005, vol. 5, No. 10, pp. 1905-1909. |
| A. V. Hatch; A. E. Herr; D. J. Throckmorton; J. S. Brennan; A. K. Singh; “Integrated Preconcentration SDS-PAGE of Proteins in Microchips Using Photo patterned Cross-Linked Polyacrylamide Gels”, Analytical Chemistry, 2006, vol. 78, pp. 4976-4984. |
| A. E. Herr; A. V. Hatch; D. J. Throckmorton; H. M. Tran; J. S. Brennan; W. V. Giannobile; A. K. Singh; “Microfludic immunoassays as rapid saliva-based clinical diagnostics”, Proceedings of the National Academy of Sciences, 2007, vol. 104, No. 13, pp. 5268-5273. |
| P. Lim; R. North; G. Vigh; “Rapid isoelectric trapping in a micropreparative-scale multicompartment electrolyzer”, Electrophoresis, 2007. vol. 28, pp. 1851-1859. |
| G. J. Sommer; A. K. Singh; A. V. Hatch; “On-Chip Isoelectric Focusing Using Photopolymerized Immobilized pH Gradients”, Analytical Chemistry, 2008, vol. 80, pp. 3327-3333. |
| Invitrogen Life Technologies, Instruction Manual, ZOOM IEF Fractionator, Cat. Nos. ZF10001 & ZF10002, Version C, Jul. 2004, pp. 1-64. |
| X. Zuo; D. W. Speicher; “A Method for Global Analysis of Complex Proteomes Using Sample Prefractionation by Solution Isoelectrofocusing Prior to Two-Dimensional Electrophoresis”, Analytical Biochemistry, 2000, vol. 284, pp. 266-278. |
| Abi-Samira, K. et al., “Infrared Controlled Waxes for Liquid-Handling and Storage on a CD-Microfluidic Platform”, The Royal Society of Chemistry, Lab Chip, 2011, pp. 723-726. |
| Albrecht, J W. et al., “Micro Free-Flow lEF Enhanced by Active Cooling and Functionalized Gels”, Electrophoresis, 2006, pp. 4960-4969, vol. 27. |
| Amersham, M. “Percoll: Methodology and Applications”, 2001, pp. 1-84. |
| Baldwin, Robert L., “How Hofmeister Ion Interactions Affect Protein Stability,” Biophysical Journal, vol. 71, Oct. 1996, pp. 2056-2063. |
| Boyko, M. et al., “Cell-Free DNA—A Marker to Predict Ischemic Brain Damage in a Rat Stroke Experimental Model,” J. Neurosura. Anesthesiol. vol. 23, No. 3, Jul. 2011, pp. 222-228. |
| Cabrera, C R. et al., “Formation of Natural pH Gradients in a Microfluidic Device under Flow Conditions: Model and Experimental Validation”, Analytical Chemistry, 2001, pp. 658-666, vol. 73. |
| Carney, J, “Rapid Diagnostic Testws Employing Latex Particles,” Analytical Proceedings, Apr. 1990, pp. 27:99-100. |
| Curtis, R.A. et al., “A Molecular Approach to Bioseparations: Protein-Protein and Proten-Salt Interactions,” Chemical Engineering Science, 2006, vol. 61, pp. 907-923. |
| Czeiger. D. et al., “Measurement of Circulating Cell-Free DNA Levels by a New Simple Fluorescent Test in Patients with Primary Colorectal Cancer,” Am. J. Olin. Pathol., 2011, vol. 135, pp. 264-270. |
| Das, C et al., “Effects of Separation Length and Voltage on Isoelectric Focusing in a Plastic Microfluidic Device”, Electrophoresis, 2006, pp. 3619-3626, vol. 27. |
| Golorkian, H. et al., “Smart-Consumables Product Development Strategy: Implications for Molecular Diagnostics”, DX Direction, 2010, 12-16. |
| Goldshtein,H., et al., “A Rapid Direct Fluorescent Assay for Cell-Free DNA Quantification in Biological Fluids,” Annals of Clinical Biochemistry, 209, vol. 46, pp. 488-494. |
| Glorikian, H. et al., “Overview of Microfluidic Applications IN IVDS”, DX Direction 1, 2010, pp. 12-16. |
| Gorg, A et al., “Recent Drvelopments in Two-Deimensional Gel Electrophoresis with Immobiliezed pH Gradients: Wide pH Gradients Up To pH 12, Longer Separation Distances and Simplified Prodedures”, electrophoresis, vol. 20, 1999, pp. 712-717 |
| Gorg, a et al., “The Current State of Two-Dimensional Electrophoresis with Immobilized pH Gradients”, Electrophoresis, vol. 21, 2000, pp. 1037-1053. |
| Herr, A E. et al., “On-Chip Coupling of Isoelectric Focusing and Free Solution Electrophoresis for Multidimensional Separations”, Analytical Chemistry, vol. 75, 2003, pp. 1180-1187. |
| Holmes, D., et al., “Leukocyte Analysis and Differntiation Using High Speed Microfluidic Singe Cell Impedance Cytometry”, Lab Chip 9, 2009, pp. 2881-2889. |
| Huang, T et al., “Microfabrication of a Tapered Channel for Isoelectric Focusing with Thermally Generated pH Gradient”, Electrophoresis, vol. 23, 2002, pp. 3504-3510. |
| International Search Report dated Dec. 24, 2009 for PCT/US2009/044550. |
| International Search Report dated Mar 1, 2012 for PCT/US2012/027299. |
| Lee, B.S., et al “A Fully Automated Immunoassay From Whole Bloon n. a Disc”; Lab Chip 9, 2009, pp. 1548-1555. |
| Lim, C.T. And Zhang, Y., “Bead-Based Microfluidic Immunoassays: The Next Generation”, Biosens. Bioelectron. 22, 20071, pp. 1197-1204. |
| Lo, C T. et al., “Photopioymerized Diffusion-Defined Ployacrylamide Gradient Gels for On-Chip Protein Sizing”, The Royal Society of Chemistry, Lab on a Chip, vol. 8, No. 8, 2008, pp. 1273-1279. |
| Lo, Y. et al., “Plasma DNA as a Prognostic Marker in Trauma Patients”, Clinical Chemistry 46:3, 2009, pp. 319-323. |
| Madou, M., et al., “Lab on a CD”; Annu. Rev. Biomed. Eng. 8, 2006, pp. 601-628. |
| Maes, M., et al., “Comparison of Sample Fixation and the Use of LDS-751 or Anti-CD45 for Leukocyte Identification in Mouse Whole Blood for Flow Cytornetry”, Journal of Immunogical Methods, 2007, p. 1-13. |
| Min J. et al., “Functional Integration of DNA Purification and Concentration into a Real Time Micro-PCR Chip,” The Royal Society of Chemistry; Lab Chip, 2011, pp. 259-265. |
| O'Farrell, P. H. , “High Resolution Two-Dimensional Electrophoresis of Proteins”, The Journal of Biological Chemistry, vol. 250, No. 9, 1975, pp. 4007-4021. |
| Price, C.P., et al., “light-Scattering Immunoassay,” Principles and Practice Immunoassay (Second Edition), 1997, Chap. 18, pp. 445-480. |
| Rhodes, A., et al., “Plasma DNA Concentration as a Predictor of Mortality and Sepsis in Critically III Patients,” Critical Care, 2006, pp. 1-7. |
| Rider, T, et al., “AB Cell-Based Sensor for Rapid Identification of Pathogens”; wwvvsciencernag.org: Science vol. 301; 2003, pp, 213-215. |
| Riegger, L., et al., “Read-Out Concepts for Multiplexed Bead-Based Flourescence Immunoassays on Centrifugal Microfluidic Platforms,” Sensors and Actuators A 125, 2006, pp. 455-462. |
| Righetti, P G. , “The Alpher, Bethe, and Gamow of IEF, the Alpha-Centaury of Electrokinetic Methodologies, Part II: Immobilized pH Gradients”, Electrophoresis, 2007, pp. 545-555, vol. 28. |
| Righetti, p. G. , “The Alpher, Bethe, Gamow of Isoelectric Focusing, the Alpha-Centaury of Electrokinetic Methodologies. Part 1”, Electrophoresis, 2006, pp. 923-938, vol. 27. |
| Satomi, T. et., al., “Design Optimization of Spirally Grooved Thrust Air Gearings for Polygon Mirrow Laser Scanners”, The Japan Society of Mechanical Engineers, 1993, Series C,, vol. 36(3), pp. 393-399. |
| Schaff, U.Y., et al., “Whole Blood Immunoassay Based on Centrifugal Bead Sedimentation,” Clinical Chemistry, 2011, vol. 57:5, pp, 753-761. |
| Tan, W et al., “Miniaturized Capillary Isoelectric Focusing in Plastic Microfludic Devices”, Electrophoresis. 2002, pp. 3638-3645, vol. 23. |
| Zhang, L., et al., “A New Biodosimetric Method: Branched DNA-Based Quantitative Detection of B1 DNA in Mouse Plasma,” The British Journal of Radiology, Aug. 3, 2010, pp. 694-701. |
| Ziegler, A. et al., “Circulating DNA: A New Diagnostic Gold Mine?” Cancer Treatment Reviews, 2002, vol. 28, pp. 255-271. |
