Method and apparatus for separating a material

Description

FIELD

The present disclosure relates to methods and apparatuses for separating biological materials, such as a selected fraction from a multiple component biological material.

BACKGROUND

This section provides background information related to the present disclosure, which is not necessarily prior art.

Various cellular or biological materials can be used to facilitate the healing or recovery process in a human patient. Selected cell types, such as stromal cells, pluripotent or multipotent stem cells, or fully differentiated cells can be applied therapeutically to the patient. For example, stem cells can be applied to an affected area of the patient, such as an area that may be damaged due to injury, chemotherapy, or radiation therapy, to assist in healing the area through differentiation of the stem cells and regeneration of the affected cells.

In performing a therapeutic procedure on a human patient using undifferentiated cells, such as stem cells or stromal cells, the undifferentiated cells can be obtained from various sources, including the patient's own anatomy. Accordingly, certain autologous cells can be applied to or injected into various portions of the patient's anatomy. Generally, a whole tissue, such as adipose tissue, or whole blood sample, can be obtained from the patient during a first procedure, selected cells can be separated from the whole tissue or blood sample, and the selected, separated cells can be reapplied to or injected into the patient during a subsequent procedure.

SUMMARY

This section provides a general summary of the disclosure, and is not a comprehensive disclosure of its full scope or all of its features.

The present teachings provide for a separation system for separating a multiple component material into at least two fractions. The separation system includes a separation device having a first end, a second end opposite to the first end, and a sidewall that extends between the first end and the second end to define a separation chamber having an interior volume. The system also includes a valve moveable between an open position and a closed position, the valve is mounted at a fixed location within the separation chamber at a position that is closer to the second end than to the first end and is spaced apart from the second end, the valve is operable to isolate a first fraction of the multiple component material having a first density on a first side of the valve from a second fraction having a second density on a second side of the valve that is opposite to the first side.

The present teachings further provide for a separation system for separating a multiple component material into at least two fractions that includes a separation device and a valve. The separation device has a first end, a second end opposite to the first end, and a sidewall that extends between the first end and the second end to define a separation chamber having an interior volume. The valve is mounted at a fixed positioned within the separation chamber at a position that is closer to the second end than to the first end and is spaced apart form the second end. The valve includes a screen, a flexible valve actuation member, and a sealing member. The flexible valve actuation member is movable in response to gravitational forces applied to the separation device. The sealing member is supported by the flexible valve actuation member. The flexible valve actuation member and the sealing member extend in a plane perpendicular to a longitudinal axis of the separation chamber and the sealing member contacts the screen to prevent the passage of materials through the screen when the valve is in a closed position. The flexible valve actuation member and the sealing member bend toward the second end when the valve is in an open position in response to gravitational forces exerted upon the separation device such that the sealing member is spaced apart from the screen to permit the passage of material through the screen.

The present teachings also provide for a method for isolating at least two fractions of a multiple component material. The method includes the following: loading the multiple component material into a separation chamber of a separation device between a valve mounted at a fixed position in the separation chamber and a first end of the device, the first end is opposite to a second end and a sidewall extends between the first end and the second end to define the separation chamber having an interior volume; centrifuging the separation device such that the valve moves to an open position in response to gravitational forces exerted on the device to permit a first fraction of the multiple component material of a first density to pass through the valve toward the second end; ceasing centrifugation of the separation device to permit the valve to move to a closed position, thus isolating the first fraction of the first density between the valve and the second end and isolating a second fraction of a second density that is less dense than the first density between the valve and the first end; and withdrawing at least one of the first fraction and the second fraction from the separation chamber for use in a subsequent procedure.

Further areas of applicability will become apparent from the description provided herein. The description and specific examples in this summary are intended for purposes of illustration only and are not intended to limit the scope of the present disclosure.

DRAWINGS

The drawings described herein are for illustrative purposes only of selected embodiments and not all possible implementations, and are not intended to limit the scope of the present disclosure.

FIG. 1 is a side view of a separation device according to the present teachings;

FIG. 2 is a side cross-sectional perspective view taken along line 2-2 of FIG. 1 illustrating a valve according to the present teachings in a closed position;

FIG. 3 is a side cross-sectional perspective view of the valve of FIG. 2 in an open position;

FIG. 4 is an exploded perspective view of the valve;

FIG. 5 is a side cross-sectional perspective view of another valve according to the present teachings;

FIG. 6 is a partially cut-away side view of the separation device being filled with a multiple component material, such as adipose tissue, for separation into at least two fractions;

FIG. 7 is a perspective view of a centrifuge for spinning the device in order to separate the multiple component material into at least two fractions, such as cellular material and purified fat when the multiple component material is adipose tissue;

FIG. 8 is a partially cut-away side view of the separation device with the valve open, thus permitting passage of at least one fraction of the multiple component material there through, such as cellular material where the multiple component material is adipose tissue;

FIG. 9 is a partially cut-away side view of the separation device showing separated fractions being extracted from the separation device;

FIG. 10 illustrates delivery of one or more of the separated fractions being delivered to a selected site in a patient;

FIG. 11 illustrates extraction of the multiple component material directly from a patient into the separation device using a vacuum pump;

FIG. 12 is similar to FIG. 11, but includes the use of a disruption chamber attached to the separation device; and

FIG. 13 is a cross-sectional view of FIG. 12 taken along line 13-13 of FIG. 12.

Corresponding reference numerals indicate corresponding parts throughout the several views of the drawings.

DETAILED DESCRIPTION

Example embodiments will now be described more fully with reference to the accompanying drawings.

With initial reference to FIGS. 1-3, a separation device in accordance with the present teachings is illustrated at reference numeral 10. The separation device 10 generally includes a first end 12, a second end 14 that is opposite to the first end 12, and a sidewall 16 that extends between the first end 12 and the second end 14. The sidewall 16 defines a separation chamber 17 of the separation device 10 having an interior volume. The sidewall 16 can be cylindrical. As illustrated, the first end 12 and the second end 14 can be positioned in spaced apart, parallel planes that are perpendicular to a longitudinal axis A of the separation chamber 17. The separation chamber 17 can have an interior volume of any suitable size, such as 90 ml, with any suitable diameter, such as 1.35 inches.

With additional reference to FIG. 4, a valve 18 is mounted at a fixed position within the separation chamber 17. Thus, the valve 18 does not move along the longitudinal axis A of the chamber 17. The valve 18 includes a grate or screen 20. The grate 20 is generally cylindrical and includes a center opening 22 with a series of radially extending spokes 24 extending therefrom. Each of the spokes 24 define an opening or passageway 25 therebetween. The spokes 24 terminate at a cylindrical outer wall 26. As illustrated, the passageways 25 are pie-shaped. However, the openings can be of any suitable shape, such as square or circular, as described below.

The grate 20 is surrounded by an annular insert 28 having a conical surface 30 that is angled toward the grate 20 to direct materials on the conical surface 30 toward the grate 20. The insert 28 has an outer diameter 32 that approximates an inner diameter of the separation chamber 17, such that no material can pass around the insert 28. The grate 20 and the opening 22 defined by the grate 20 provide support and alignment for a second extraction tube 72, which is further described herein. In place of the grate 20, any suitable screen with or without an opening therein can be used. Further, the grate 20 may be optional and the device 10 can be provided with the grate 20 removed and an opening provided in its place.

The valve 18 further includes a sealing member 34 and a support or valve actuation member 36. As illustrated, the sealing member 34 and the valve actuation member 36 can be aligned along the longitudinal axis A of the separation chamber 17. The sealing member 34 is generally shaped as a cylindrical disk and includes an opening 38 at its axial center. The sealing member 34 can be made of any suitable material, including a flexible material, such as a silicone rubber material. The sealing member 34 is sized to seal the plurality of passageways 25.

The valve actuation member 36 can include a cylindrical disk 40 and a mounting tube 42 extending therefrom along a longitudinal axis of the valve actuation member 36. The cylindrical disk 40 has a circumference that is substantially similar to that of the sealing member 34. The cylindrical disk 40 includes an opening 44 at its axial center. As further described herein, the cylindrical disk 40 provides support for the sealing member 34 to position the sealing member 34 against the grate 20 and prevent the passage of materials through the passageways 25 when the valve 18 is in the closed position. Further, the cylindrical disk 40 is flexible in response to gravitational forces, such as those experienced during centrifugation, to move the sealing member 34 from contact with the grate 20 and permit the passage of materials through the passageways 25 when the valve 18 is in the open position.

The mounting tube 42 extends from the cylindrical disk 40 along the axial center of the cylindrical disk. The mounting tube 42 has a circumference that is generally smaller than the circumference of the cylindrical disk 40. Proximate to a distal end 46 of the mounting tube 42 is at least one aperture 48. As illustrated, the distal end 46 includes four of the apertures 48, which are spaced evenly about the mounting tube 42 at approximately 90° intervals. A through port 50 extends between the apertures 48 and the opening 44 to provide fluid communication through the valve actuation member 36.

The cylindrical disk 40 of the valve actuation member 36 can be formed of any suitable material that can flex when a force is applied to it, such as a centrifugal force or a pressure differential force. For example, the disk 40 can be any resilient member operable to bias the valve 18 in a closed position such that the sealing member 34 blocks the passage of materials through the passageways 25. Material selected for the cylindrical disk 40 can include acrylic, polycarbonate, and any other appropriate resilient, flexible, and substantially inert material. The sealing member 34 can be mounted to the cylindrical disk 40 in any suitable manner, such as by using a suitable adhesive. Alternatively, the sealing member 34 can be a coating on the disk 40 and/or integral with the disk 40. The sealing member 34 can also be a separate component that is not secured to the disk 40, but rather sits thereon and is supported by the disk 40.

The assembled valve 18 is positioned within the separation chamber 17 such that the distal end 46 of the mounting tube 42 abuts the second end 14 of the chamber 17, which may include a funnel 52 as further described herein. The grate 20, the sealing member 34, and the valve actuating member 36, are each positioned such that the center opening 22, the opening 38, and the opening 44 respectively are all aligned along the longitudinal axis A. When the valve is in the closed position as illustrated in FIG. 2, the cylindrical disk 40 supports the sealing member 34 against the grated portion 20 of the insert 28 to block and seal the passage of materials through the passageways 25 or openings defined by the spokes 24. The insert 28 including the grate 20 can be fixedly mounted within the separation chamber 17 using any suitable fastening device, method or system. For example, the insert 28 can be mounted to an interior of the sidewall 16 using a suitable adhesive or a press fit.

With additional reference to FIG. 3, the valve 18 is illustrated in an open position. In the open position, the cylindrical disk 40 is not perpendicular to the longitudinal axis A of the separation chamber 17, as it is in the open position, but rather its perimeter is flexed downward toward the second end to space the sealing member 34 apart from the grate 20 and permit the passage of materials through the openings 25 between the spokes 24. As further described herein, movement of the cylindrical disk 40 between the closed position of FIG. 2, for example, and the open position of FIG. 3, for example, can be caused by centrifugal force or pressure exerted against the sealing member 34 and the cylindrical disk 40 when the separation chamber 17 is loaded with a multiple component composition and inserted in a centrifuge.

The funnel 52 at the second end 14 of the chamber 17 generally includes a base portion 54 at the longitudinal axis A of the separation chamber 17. Extending from the base portion 54 is an angled cylindrical sidewall 56. The sidewall 56 is angled such that it slopes from the sidewall 16 of the separation chamber 17 toward the base portion 54. Thus, the funnel 52 directs material along the angled cylindrical sidewall 56 toward the base portion 54 where the apertures 48 of the mounting tube 42 are positioned. The funnel 52 can be secured at the second end 14 in any suitable manner, such as with a suitable adhesive or a press fit. The funnel 52 can include a counterbore or recess 55 on its undersurface facing the second end 14 of the device 10. The recess 55 accommodates a dimple 57 at the second end 14 of the device 10. Cooperation between the dimple 57 and the recess 55 can retain the funnel 52 centered in the separation chamber 17. The dimple 57 can cooperate with a corresponding feature in a centrifugation device to properly position the device 10 in the centrifuge.

The separation chamber further includes a loading port 58, a first extraction port 60, and a second extraction port 62. The loading port 58 can be any suitable port that extends into the separation chamber 17 to permit the introduction of materials into the separation chamber 17. As illustrated, the loading port 58 is at the first end 12 and extends there through. The loading port 58 can also be offset from the longitudinal axis A, as illustrated. The loading port 58 can include a loading port cap 64 that can be fastened to the port 58 using any suitable connection, such as a Luer lock connection. The Luer lock connection can also cooperate with a device for delivering the multiple component material to the separation chamber 17, such a syringe.

The first extraction port 60 can be any suitable port that extends into the separation chamber 17 to permit the withdrawal of one or more components of a multiple component material from within the separation chamber 17. As illustrated, the first extraction port 60 is at the first end 12 and extends there through. The first extraction port 60 can include a cap 66 that can be fastened to the first extraction port 60 using any suitable connection, such as a Luer lock connection. The Luer lock connection can also cooperate with a device for withdrawing the components from within the separation chamber 17, such as a syringe. Extending from the first extraction port 60 can be a first extraction tube 68. As illustrated, the first extraction tube 68 extends from the port 60 to a position proximate to a first side 69 of the valve 18 that faces the first end 12. However, one skilled in the art will recognize that the extraction tube 68 can be of any suitable length to extract a desired component of the multiple component composition of a specific density. For example, if the composition includes adipose tissue and purified fat is desired for extraction, then the extraction tube 68 can extend approximately 1.5 inches from the first end 12, such as in applications where 60 ml of adipose tissue is loaded for separation in the separation chamber 17 having a diameter of about 1.35 inches and a volume of about 90 ml. This is because purified fat is typically one of the least dense fractions of adipose tissue. Alternatively, if one or more of the more dense fractions of adipose tissue is desired for extraction, such as oil or excess/tumescent fluid, then the extraction tube 68 can extend from the first end 12 to a distance that is about 0.25 inches from the valve 18. Such a longer extraction tube 68 can also be use to extract purified fat by drawing off the more dense fractions prior to drawing the purified fat.

The second extraction port 62 can be any suitable port that extends into the separation chamber 17 to permit the withdrawal of one or more components of the multiple component material from within the separation chamber 17. As illustrated, the second extraction port 62 is at the first end 12 and extends there through. The second extraction port 62 can include a cap 70 that can be fastened to the second extraction port 62 using any suitable connection, such as a Luer lock connection. The Luer lock connection can also cooperate with a device for withdrawing the components from within the separation chamber 17, such as a syringe.

Extending from the second extraction port 62 can be the second extraction tube 72. As illustrated, the second extraction tube 72 extends from the second extraction port 62 along the longitudinal axis A to the valve 18. At the valve 18, the second extraction tube 72 extends through the center opening 22 of the grate 20, through the opening 38 of the sealing member 34, through the opening 44 of the valve actuation member 36, and the through port 50 to a position proximate to the apertures 48. Thus, the second extraction tube 72 provides fluid communication between the apertures 48 and the second extraction port 62. The second extraction tube 72 can sit on a shoulder 73 of the mounting tube 42 and can be secured within the valve 18, such as within the through port 50, in any suitable manner, such as with a press-fit or a suitable adhesive.

One skilled in the art will appreciate that the grate or screen 20 can be provided in a variety of different configurations in addition to those illustrated. Accordingly and with additional reference to FIG. 5, the grate or screen 20 can include round cutouts 74 in place of the spokes 24. Any other shaped opening or cutout can also be used that will permit passage of select fractions of a multiple component material.

With additional reference to FIGS. 6-9, use of the separation device 10 to separate adipose tissue into different fractions including cellular material, purified fat, and tumescent fluid is described below. This description is for exemplary purposes only because the separation device 10 can be used to separate fractions of a wide variety of different multiple component materials.

With initial reference to FIG. 6, the multiple component composition, such as adipose tissue, is loaded into the separation chamber 17 through the loading port 58. The adipose tissue can be delivered to the separation chamber 17 using any suitable transfer device, such as a syringe 80. The adipose tissue is loaded with the valve 18 in the closed position of FIG. 2. Thus, the adipose tissue will initially be seated atop the valve 18 on the first side 69 of the valve 18 proximate to the first end 12. Any suitable amount of adipose tissue can be used, such as about 60 ml. when a 90 ml. separation chamber having a diameter of 1.35 inches is used.

Prior to being loaded in the separation chamber 17, the adipose tissue, or any multiple component composition, can be optionally subject to mechanical disruption. Mechanical disruption loosens the adipose tissue to facilitate separation of the different fractions during further processing. Any suitable disruptor can be used, such as the disruptors described in U.S. application Ser. No. 12/395,085 titled “A System For Separating A Material,” which was filed on Feb. 27, 2009 and is assigned to Biomet Biologics, LLC., which is incorporated by reference herein. This type of disruptor includes a screen or grate that the multiple component material is forced through to loosen the interaction between the different fractions.

After the adipose tissue is loaded, a suitable anticoagulant, such as citrate phosphate dextrose (“CPD”), can be added as well as through the loading port 58. Any suitable amount of CPD can be added, such as about 8.5 cc for 60 cc of adipose tissue. The separation device 10 can then be incubated at about 37° C. for about five minutes. Any suitable device or method can be used to perform the incubation, such as by placing the separation device 10 in a heat bath or wrapping the device 10 in a heat pack.

The separation device 10 containing the adipose tissue is then spun in a suitable rotational device, such as the centrifuge 90 illustrated in FIG. 7. As illustrated, multiple separation devices 10 can be spun simultaneously. The separation device 10 can be initially spun at about 100 to about 1,500× gravity for about 5 minutes to allow for initial separation of fat layers, including oil, fatty tissue, excess/tumescent fluid, etc. The speed of the centrifuge can then increased to about 1,500 to about 3,000× gravity for about an additional 12-15 minutes. Alternatively, the separation device 10 can be subject to a single centrifugation at about 1,500 to about 3,000× gravity and 3,200 revolutions/minute for about 15 minutes.

During centrifugation, gravitational forces act on the valve 18 to cause the valve 18 to move to the open position of FIG. 3. Specifically and with additional reference to FIG. 8, gravitational forces cause the valve actuation member 36 and the sealing member 34 mounted thereto to bend downward along the longitudinal axis A such that the outer diameter of both the valve actuation member 36 and the sealing member 34 move toward the second end 14. The valve actuation member 36 and the sealing member 34 bend at the portions proximate to the longitudinal axis A to provide a “flap valve.” This separates the sealing member 34 from the grate 20 to create a space therebetween through which components of the multiple component composition, such as cellular material where the multiple component material is adipose tissue, can pass and collect at the base portion 54 of the insert 52, which along with the angled cylindrical sidewall 56 defines a sump on a second side 71 of the valve 18.

With additional reference to FIG. 9, centrifugation causes the different fractions of the multiple component material to separate according to density such that fractions with the greatest density settle at the second end 14. The least dense fractions settle proximate to the first end 12 or most distal to the second end 14. After centrifugation, the valve 18 returns to the closed position, illustrated in, for example, FIG. 9. When closed, the valve 18 separates the multiple component material such that at least one fraction of a first density is separated between the valve 18 and the second end 14, and a second fraction having a second density that is greater than the first density is separated on an opposite side of the valve 18, which is proximate to the first end 12.

The valve 18 is positioned within the separation chamber 17 along the longitudinal axis A such that after centrifugation the two fractions of the multiple component material that are most desirable are separated on opposite sides of the valve 18. One skilled in the art will recognize that the position of the valve 18 along the longitudinal axis A will depend on the densities of the most desired fractions.

For example, when the multiple component material is adipose tissue, the valve can be positioned from about 0.5 inches to about 1.5 inches, such as about 0.75 inches, from the second end 14 in applications where the separation chamber 17 has a diameter of about 1.35 inches and a volume of about 90 ml. As a result, the fractions of adipose tissue of the greatest density, including cellular material 92 having a typical density of about 1.06 g/ml to about 1.1 g/ml, will be isolated proximate to the second end 14 on the second side 71 of the valve 18. Conversely, the fractions of adipose tissue of the least density, including purified fat having a density of about 0.95 g/ml, excess water or other fluid having a density of about 1.0 g/ml, oil, etc. at 94 are isolated on the first side 69 of the valve 18. A tumescent fluid layer 95 will be isolated on both sides of the valve 18 between the cellular material 92 and the purified fat.

To provide higher cell yields, the diameter of the separation chamber 17 can be increased and/or the volume of adipose tissue can be decreased. This increases the surface area of the adipose tissue, thus making it easier for the cells to travel through the fat and extra cellular matrix (ECM) toward the second end 14.

Increased cell yields can also be provided by subjecting the fractions 94 isolated on the first side 69 of the valve 18, such as purified fat, excess fluid, oil, etc., to a second disruption and/or centrifugation process. For example, after the one or more fractions 94 are isolated through centrifugation, the fractions 94 can again be passed through the disruptor 120 to loosen the interaction between the materials and then again be centrifuged in the separation chamber 17 to permit isolation of cellular material 94 on the second side 71 of the valve 18 that was not previously isolated. Both the disruption and centrifugation processes are further described below.

With additional reference to FIG. 9, the isolated fractions can be withdrawn as desired using a suitable extraction device, such as a syringe. For example, the purified fat, excess fluid, oil, etc. 94 can be withdrawn through the first extraction port 60 using a suitable syringe 96. Similarly, the cellular material 92 can be withdrawn through the second extraction port 62, via the aperture 48 and the second extraction tube 72 using a suitable syringe 98. The angled cylindrical sidewall 56 and the base portion 54 act as a sump to direct the cellular material 92 toward the apertures 48 of the distal end 46 of the mounting tube 42 to facilitate withdrawal of the cellular material 92 through the second extraction port 62. Prior to withdrawing the purified fat through the first extraction port 60 and subsequent to withdrawing the cellular material 92 through the second extraction port 62, the tumescent fluid layer 95 can be withdrawn through the first and the second extraction ports 60 and 62.

The isolated fractions can be used for a variety of different purposes. For example, the cellular material 92 can be used to facilitate wound healing, such as by directly injecting the cellular material 92 to a wound site of a patient 100, as illustrated in FIG. 10. The purified fat can be used in a variety of different types of reconstructive and cosmetic surgery, such as facial reconstruction, breast reconstruction, and in most any area in which a fat filling is desired.

With additional reference to FIG. 11, a suction tube 102 with a suitable impingement device attached to an end thereof, such as a cannula 104, can be used to draw the multiple component material directly from a patient into the separation device 10. The end of the suction tube 102 opposite to the cannula 104 can be secured to the loading port 58 using any suitable connection, such as a Luer lock. The cannula 104 can be inserted directly into an area 106 of the patient from where the adipose tissue is desired to be removed.

To facilitate withdrawal of the adipose tissue from the desired area 106 of the patient, a suitable extraction device, such as a vacuum pump 110, can be used. The vacuum pump 110 can be connected to a separate vacuum port 112 at the first end 12 of the separation chamber 17 that provides fluid communication with the interior volume of the separation chamber 17. The vacuum pump 110 can be connected to the vacuum port 112 using a suitable suction tube 108. The vacuum pump 110 can be any suitable vacuum pump 110 operable to withdraw the multiple component material out of the suitable area 106 of the patient to within the separation chamber 17. After the multiple component composition is drawn into the separation chamber 17, the vacuum pump 110 can be disconnected from the vacuum port 112 and the vacuum port 112 can be closed with a suitable cap.

With additional reference to FIG. 12, the separation device 10 can include a suitable disruptor, such as the disruptor 120. The disruptor 120 generally includes a disruptor chamber 122, a plunger 124, a disruptor inlet port 126, a disruptor vacuum port 128, a disruption screen 130, and a disruptor outlet port 132.

The disruptor inlet port 126 provides fluid communication between an exterior of the disruptor 120 and the disruptor chamber 122. The suction tube 102 with the cannula 104 attached thereto can be connected to the disruptor inlet port 126 using any suitable connection, such as a Luer lock connection.

The disruptor vacuum port 128 also provides fluid communication between an exterior of the disruptor 120 and the disruptor chamber 122. The vacuum pump 110 can be connected to the disruptor vacuum port 128 using any suitable connection, such as a Luer lock connection, to draw the multiple component composition into the disruptor chamber 122.

After a suitable amount of the multiple component material, such as adipose tissue, is drawn into the chamber 122, the pump 110 can be stopped and the plunger 124 can be depressed to drive the multiple component material through the disruption screen 130, which is also illustrated in FIG. 13. The disruption screen 130 can be any suitable disruption screen known in the art, such as those described in U.S. application Ser. No. 12/395,085 incorporated by reference herein. As illustrated, the disruption screen 130 includes a plurality of round openings 131, however any suitably shaped openings or grated surface can be provided to disrupt a material to be passed therethrough. As the material is pushed through the disruption screen, it is softened and its fractions are loosened to facilitate separation of the fractions during the centrifugation process.

The disruptor outlet port 132 is connected to an inlet port 134 of the separation device 10. As illustrated, the inlet port 134 extends through the first end 12 and is similar to the loading port 58. The inlet port 134 can be connected to the disruptor outlet port 132 in any suitable manner, such as through a Luer lock connection, to provide fluid communication between the disruptor chamber 122 and the interior volume of the separation chamber 17. Thus, as the plunger 124 is depressed, the multiple component composition is pushed through the disruptor screen 130 and into the interior volume of the separation chamber 17 where it is separated into its different fractions through centrifugation as described above. The separate inlet port 134 for the disruptor 120 is optional as the disruptor 120 can also be connected to the loading port 58.

The inlet port 134 can be located at the axial center A of the first end 12 to facilitate introduction of the adipose tissue into the separation chamber 17, however, the inlet port 134 can be located at any suitable location and can be eliminated altogether because the disruptor 120 can also be connected to the loading port 58. When the inlet port 134 is located at the axial center A, the second extraction port 62 can be moved offset from the axial center A. Accordingly, the second extraction tube 72 does not extend entirely along the axial center A as described above, but can be offset with an elbow portion 136. The inlet port 134 can be in addition to, or can take the place of, the loading port 58.

While the disruptor screen 130 is illustrated as being integral with the disruptor 120, the disruptor screen 130 can also be a separate component that is connected to both the disruptor inlet port 126 and the disruptor 120 using suitable fastening devices, such as Luer lock connections. Further, the disruptor screen 130 can be integral with the separation device 10 and the disruptor 120 can be connected to the disruptor screen 130 with a suitable connection.

While the disruptor 120 is illustrated as being connected to a single separation device 10, the disruptor 120 can be connected to multiple separation devices 10 through the use of a suitable connection device, such as a branch connector, that will provide fluid communication between the disruptor 120 and inlet ports of multiple separation chambers.

The present teachings further provide for a sterile method of using the separation device 10. With reference to FIGS. 11 and 12, the cannula 104 and the suction tube 102 can be sterilized and passed into a sterile field where the cannula 104 can be connected to a first end of the suction tube 102. A second end of the suction tube 102 can be connected to either the loading port 58 of the separation device 10 (FIG. 11) or the disruptor inlet port 126 of the disruptor 120 (FIG. 12). The separation device 10 and the disruptor 120 may be inside or outside of the sterile field depending on the procedure. The suction tube 108 is then connected to the vacuum pump 110, which is outside of the sterile field, and either the first extraction port 60 (FIG. 11) or the disruptor vacuum port 128 (FIG. 12). Thus, the separation device 10 need not ever enter the sterile field, thus allowing it to be handled by non-sterile personnel for processing in the centrifuge 90. Use of the device 10 outside of the sterile field is advantageous because it frees up space in the sterile area. Use of the device 10 inside of the sterile area decreases the possibility of contamination.

To facilitate collection of the multiple component composition, multiple cannulas 104 can be inserted into area 106 of the patient from where the composition is to be removed and multiple suction tubes 102 can be connected to the cannulas 104. The suction tubes 102 can then be connected to the loading port 58 or the disruptor inlet port 126 using a suitable connecting device, such as a suitable branch connector. Also, multiple vacuum pumps 110 can be used to increase the vacuum force. The pumps 110 can be connected to the first extraction port 60 or the disruptor vacuum port 128 using multiple suction tubes 108 connected by, for example, a branch line.

The foregoing description of the embodiments has been provided for purposes of illustration and description. It is not intended to be exhaustive or to limit the invention. Individual elements or features of a particular embodiment are generally not limited to that particular embodiment, but, where applicable, are interchangeable and can be used in a selected embodiment, even if not specifically shown or described. The same may also be varied in many ways. Such variations are not to be regarded as a departure from the invention, and all such modifications are intended to be included within the scope of the invention.

Claims

1. A separation system for separating a multiple component material into at least two fractions comprising: a separation device having a first end, a second end opposite to the first end, and a sidewall that extends between the first end and the second end to define a separation chamber having an interior volume; anda valve moveable between an open position and a closed position, the valve is mounted at a fixed location within the separation chamber at a position that is closer to the second end than to the first end and is spaced apart from the second end, the valve is operable to isolate a first fraction of the multiple component material having a first density on a first side of the valve from a second fraction having a second density on a second side of the valve that is opposite to the first side,wherein the valve includes a screen, a valve activation member, and a seal, each of the screen, the valve activation member, and the seal define a through hole at an axial center thereof;wherein the through hole is in fluid communication with apertures at an end of the valve activation member proximate to the second end; andwherein an extraction tube is seated in the through hole and is connected to an extraction port of the separation device.
2. The separation system of claim 1, further comprising a sump base having angled walls at the second end of the separation device, the valve is between the first end of the separation device and the sump base.
3. The separation system of claim 1, wherein the valve includes an insert having a conical surface that extends between the sidewall and a longitudinal axis of the separation chamber, the conical surface is angled downward toward the second end of the separation chamber.
4. The separation system of claim 1, wherein the screen defines openings that are one of circular and pie-shaped.
5. The separation system of claim 1, wherein the seal that is one of the following: fastened to the activation member, integral with the activation member, and separate from the activation member.
6. The separation system of claim 5, wherein the valve activation member is movable between a closed position and an open position, in the closed position the valve activation member and the seal extend along a plane that is perpendicular to a longitudinal axis of the separation chamber and the seal contacts a grated portion of the valve to prevent the passage of material through the screen, in the open position the valve activation member and the seal are flexed toward the second end and the seal is spaced apart from the grated portion of the screen to permit the passage of material through the valve.
7. The separation system of claim 1, further comprising a disruptor and a vacuum pump in communication with the separation chamber.
8. The separation system of claim 1, wherein the multiple component material includes adipose tissue; wherein the first fraction is isolated between the valve and the second end, the first fraction includes cellular material;wherein the second fraction is isolated between the valve and the first end, the second fraction includes fat; andwherein a third fraction is isolated between the valve and the first fraction and between the valve and the second fraction, the third fraction includes tumescent fluid.
9. A separation system for separating a multiple component material into at least two fractions comprising: a separation device having a first end, a second end opposite to the first end, and a sidewall that extends between the first end and the second end to define a separation chamber having an interior volume; anda valve mounted at a fixed positioned within the separation chamber at a position that is closer to the second end than to the first end and is spaced apart from the second end, the valve includes: a screen;a flexible valve actuation member that is movable in response to gravitational forces applied to the separation device; anda sealing member supported by the flexible valve actuation member;wherein each of the screen, the flexible valve actuation member, and the sealing member define a through hole at an axial center thereof;wherein the through hole is in fluid communication with apertures at an end of the valve activation member proximate to the second end; andwherein an extraction tube is seated in the through hole and is connected to an extraction port of the separation device;wherein the flexible valve actuation member and the sealing member extend in a plane perpendicular to a longitudinal axis of the separation chamber and the sealing member contacts the screen to prevent the passage of materials through the screen when the valve is in a closed position; andwherein the flexible valve actuation member and the sealing member bend toward the second end when the valve is in an open position in response to gravitational forces exerted upon the separation device such that the sealing member is spaced apart from the screen to permit the passage of material through the screen.
10. The separation system of claim 9, wherein the valve is operable to isolate a first fraction of the multiple component material having a first density on a first side of the valve from a second fraction having a second density on a second side of the valve that is opposite to the first side, and the valve is operable to isolate a third fraction including tumescent fluid between the valve and the first fraction and between the valve and the second fraction.
11. The separation system of claim 9, further comprising a second extraction tube extending from a position that is proximate to a side of the valve facing the first end to a second extraction port of the separation chamber.
12. The separation system of claim 9, further comprising a disruptor and a vacuum pump in fluid communication with the separation chamber.
13. The separation system of claim 9, wherein, with adipose tissue present in the separation chamber, the valve moves to the open position when the device is spun to permit cellular material to pass through the valve; and wherein after the device is spun the valve moves to the closed position to isolate the cellular material between the valve and the second end, the cellular material can be withdrawn from the separation device for further use.
14. The separation system of claim 9, wherein the screen, the flexible valve, and the sealing member are aligned along a longitudinal axis of the separation chamber.
15. A method for isolating at least two fractions of a multiple component material comprising: loading the multiple component material into a separation chamber of a separation device between a valve mounted at a fixed position in the separation chamber and a first end of the device, the first end is opposite to a second end and a sidewall extends between the first end and the second end to define the separation chamber having an interior volume;wherein each of the screen, the flexible valve actuation member, and the sealing member define a through hole at an axial center thereof;wherein the through hole is in fluid communication with apertures at an end of the valve activation member proximate to the second end; andwherein an extraction tube is seated in the through hole and is connected to an extraction port of the separation device;centrifuging the separation device such that the valve moves to an open position in response to gravitational forces exerted on the device to permit a first fraction of the multiple component material of a first density to pass through the valve toward the second end;ceasing centrifugation of the separation device to permit the valve to move to a closed position, thus isolating the first fraction of the first density between the valve and the second end and isolating a second fraction of a second density that is less dense than the first density between the valve and the first end; andwithdrawing at least one of the first fraction and the second fraction from the separation chamber for use in a subsequent procedure.
16. The method of claim 15, further comprising loading adipose tissue into the separation chamber to isolate the first fraction including cellular material, the second fraction including purified fat, and a third fraction including tumescent fluid; incubating the separation device with the adipose tissue loaded therein for about five minutes at about 37° C.; andcentrifuging the device at a speed of about 3,200 revolutions/minute for about fifteen minutes.
17. The method of claim 15, further comprising extracting the multiple component material from a patient and simultaneously loading the material directly into the separation device using a vacuum pump.
18. The method of claim 15, further comprising subjecting the multiple component material to disruption prior to loading the multiple component material into the separation chamber.

US Referenced Citations (486)

Number	Name	Date	Kind
280820	Hickson et al.	Jul 1883	A
593333	Park	Nov 1897	A
1468313	Lux	Sep 1923	A
1593814	Vogel	Jul 1926	A
2722257	Lockhart	Nov 1955	A
3013557	Pallotta	Dec 1961	A
3159159	Cohen	Dec 1964	A
3409165	Creith	Nov 1968	A
3441143	Kudlaty	Apr 1969	A
3453364	Flodin et al.	Jul 1969	A
3469369	Helmke	Sep 1969	A
3508653	Coleman	Apr 1970	A
3545671	Ross	Dec 1970	A
3583627	Wilson	Jun 1971	A
3596652	Winkelman	Aug 1971	A
3654925	Holderith	Apr 1972	A
3706305	Berger et al.	Dec 1972	A
3706306	Berger et al.	Dec 1972	A
3723244	Breillatt, Jr.	Mar 1973	A
3779383	Ayres	Dec 1973	A
3785549	Latham, Jr.	Jan 1974	A
3814248	Lawhead	Jun 1974	A
3849072	Ayres	Nov 1974	A
3850369	Bull et al.	Nov 1974	A
3879295	Glover et al.	Apr 1975	A
3887466	Ayres	Jun 1975	A
3894952	Ayres	Jul 1975	A
3896733	Rosenberg	Jul 1975	A
3897337	Ayres	Jul 1975	A
3897343	Ayres	Jul 1975	A
3909419	Ayres	Sep 1975	A
3929646	Adler	Dec 1975	A
3931010	Ayres et al.	Jan 1976	A
3931018	North, Jr.	Jan 1976	A
3935113	Ayres	Jan 1976	A
3937211	Merten	Feb 1976	A
3941699	Ayres	Mar 1976	A
3945928	Ayres	Mar 1976	A
3951801	Ayres	Apr 1976	A
3957654	Ayres	May 1976	A
3962085	Liston et al.	Jun 1976	A
3965889	Sachs	Jun 1976	A
3972812	Gresl, Jr.	Aug 1976	A
3982691	Schlutz	Sep 1976	A
4001122	Griffin	Jan 1977	A
4020831	Adler	May 1977	A
4046699	Zine, Jr.	Sep 1977	A
4055501	Cornell	Oct 1977	A
4059108	Latham, Jr.	Nov 1977	A
4066549	Oeser et al.	Jan 1978	A
4077396	Wardlaw et al.	Mar 1978	A
4088582	Murty et al.	May 1978	A
4146172	Cullis et al.	Mar 1979	A
4152270	Cornell	May 1979	A
4154690	Ballies et al.	May 1979	A
4159896	Levine et al.	Jul 1979	A
4187979	Cullis et al.	Feb 1980	A
4203840	Stoeppler et al.	May 1980	A
4204537	Latham, Jr.	May 1980	A
4225580	Rothman et al.	Sep 1980	A
4269718	Persidsky	May 1981	A
4294707	Ikeda et al.	Oct 1981	A
4298598	Schwarz et al.	Nov 1981	A
4300717	Latham, Jr.	Nov 1981	A
4303193	Latham, Jr.	Dec 1981	A
4314823	Rich, Jr. et al.	Feb 1982	A
4322298	Persidsky	Mar 1982	A
4362567	Schwarz et al.	Dec 1982	A
4364832	Ballies et al.	Dec 1982	A
4377572	Schwarz et al.	Mar 1983	A
4379849	Heimreid	Apr 1983	A
4411794	Schwinn et al.	Oct 1983	A
4414976	Schwarz et al.	Nov 1983	A
4416654	Schoendorfer et al.	Nov 1983	A
4417981	Nugent	Nov 1983	A
4424132	Iriguchi et al.	Jan 1984	A
4427650	Stroetmann et al.	Jan 1984	A
4427651	Stroetmann et al.	Jan 1984	A
4442655	Stroetmann et al.	Apr 1984	A
4443345	Wells	Apr 1984	A
4446021	Aufderhaar et al.	May 1984	A
4453927	Sinko	Jun 1984	A
4453939	Zimmerman et al.	Jun 1984	A
4464167	Schoendorfer et al.	Aug 1984	A
4511662	Baran et al.	Apr 1985	A
4537767	Rothman et al.	Aug 1985	A
RE32089	Blatt et al.	Mar 1986	E
4577514	Bradley et al.	Mar 1986	A
4610656	Mortensen	Sep 1986	A
4617009	Ohlin et al.	Oct 1986	A
4627879	Rose et al.	Dec 1986	A
4631055	Redl et al.	Dec 1986	A
4632761	Bowers et al.	Dec 1986	A
4639316	Eldegheidy	Jan 1987	A
4650678	Fuhge et al.	Mar 1987	A
4655211	Sakamoto et al.	Apr 1987	A
4672969	Dew	Jun 1987	A
4675117	Neumann et al.	Jun 1987	A
4680025	Kruger et al.	Jul 1987	A
4714457	Alterbaum	Dec 1987	A
4735616	Eibl et al.	Apr 1988	A
4735726	Duggins	Apr 1988	A
4755300	Fischel et al.	Jul 1988	A
4755301	Bowers	Jul 1988	A
4770779	Ichikawa et al.	Sep 1988	A
4776964	Schoendorfer et al.	Oct 1988	A
4818291	Iwatsuki et al.	Apr 1989	A
4818386	Burns	Apr 1989	A
4828710	Itoh et al.	May 1989	A
4832851	Bowers et al.	May 1989	A
4844818	Smith	Jul 1989	A
4846835	Grande	Jul 1989	A
4850952	Figdor et al.	Jul 1989	A
4853137	Ersson et al.	Aug 1989	A
4871462	Fischel et al.	Oct 1989	A
4874368	Miller et al.	Oct 1989	A
4877520	Burns	Oct 1989	A
4879031	Panzani et al.	Nov 1989	A
4902281	Avoy	Feb 1990	A
4909251	Seelich et al.	Mar 1990	A
4915847	Dillon et al.	Apr 1990	A
4917801	Luderer et al.	Apr 1990	A
4928603	Rose et al.	May 1990	A
4929242	Desecki et al.	May 1990	A
4939081	Figdor et al.	Jul 1990	A
4943273	Pages et al.	Jul 1990	A
4946601	Fiehler	Aug 1990	A
4957637	Cornell	Sep 1990	A
4957638	Smith	Sep 1990	A
4983157	Pober et al.	Jan 1991	A
4983158	Headley	Jan 1991	A
4985153	Kuroda et al.	Jan 1991	A
5000970	Shanbhag et al.	Mar 1991	A
5002571	O'Donnell, Jr. et al.	Mar 1991	A
5019243	McEwen et al.	May 1991	A
5024613	Vasconcellos et al.	Jun 1991	A
5030215	Morse et al.	Jul 1991	A
5030341	McEwen et al.	Jul 1991	A
5039401	Columbus et al.	Aug 1991	A
5045048	Kaleskas et al.	Sep 1991	A
5047004	Wells	Sep 1991	A
5053127	Schoendorfer et al.	Oct 1991	A
5053134	Luderer et al.	Oct 1991	A
5071570	Shiraki et al.	Dec 1991	A
5080262	Herold et al.	Jan 1992	A
5086784	Levine et al.	Feb 1992	A
5100564	Pall et al.	Mar 1992	A
5104375	Wolf et al.	Apr 1992	A
5112484	Zuk, Jr.	May 1992	A
5112490	Turpen	May 1992	A
5131907	Williams et al.	Jul 1992	A
5137832	Levine et al.	Aug 1992	A
5141645	Shiraki et al.	Aug 1992	A
5147290	Jonsson et al.	Sep 1992	A
5152905	Pall et al.	Oct 1992	A
5156613	Sawyer	Oct 1992	A
5165938	Knighton	Nov 1992	A
5171456	Hwang et al.	Dec 1992	A
5173295	Wehling et al.	Dec 1992	A
5178602	Wells	Jan 1993	A
5185001	Galanakis	Feb 1993	A
5190057	Sarfarazi	Mar 1993	A
5190759	Lindblad et al.	Mar 1993	A
5197985	Caplan et al.	Mar 1993	A
5203825	Haynes et al.	Apr 1993	A
5204537	Bennet et al.	Apr 1993	A
5206023	Hunziker et al.	Apr 1993	A
5207638	Choksi et al.	May 1993	A
5217426	Bacehowski et al.	Jun 1993	A
5217627	Pall et al.	Jun 1993	A
5219328	Morse et al.	Jun 1993	A
5226877	Epstein	Jul 1993	A
5226914	Caplan et al.	Jul 1993	A
5234608	Duff	Aug 1993	A
5236604	Fiehler	Aug 1993	A
5251786	Sarrine	Oct 1993	A
5258126	Pall et al.	Nov 1993	A
5260420	Burnouf-Radosevich et al.	Nov 1993	A
5269927	Fiehler	Dec 1993	A
5271852	Luoma, II	Dec 1993	A
5279825	Wehling et al.	Jan 1994	A
5281342	Biesel et al.	Jan 1994	A
5290552	Sierra et al.	Mar 1994	A
5290918	Bui-Khac et al.	Mar 1994	A
5298171	Biesel et al.	Mar 1994	A
5304372	Michalski et al.	Apr 1994	A
5316674	Pall et al.	May 1994	A
5318524	Morse et al.	Jun 1994	A
5318782	Weis-Fogh et al.	Jun 1994	A
5321126	van Dommelen et al.	Jun 1994	A
5322620	Brown et al.	Jun 1994	A
5330974	Pines et al.	Jul 1994	A
5344752	Murphy	Sep 1994	A
5354483	Furse	Oct 1994	A
5370802	Brown	Dec 1994	A
5372945	Alchas et al.	Dec 1994	A
5376263	Fischel	Dec 1994	A
5387187	Fell et al.	Feb 1995	A
5393674	Levine et al.	Feb 1995	A
5395923	Bui-Khac et al.	Mar 1995	A
5403272	Deniega et al.	Apr 1995	A
5405607	Epstein	Apr 1995	A
5409833	Hu et al.	Apr 1995	A
5411885	Marx	May 1995	A
5417650	Gordon	May 1995	A
5420250	Lontz	May 1995	A
5443481	Lee	Aug 1995	A
5454958	Fiehler	Oct 1995	A
5456693	Conston et al.	Oct 1995	A
5456885	Coleman et al.	Oct 1995	A
5474687	Van Vlasselaer	Dec 1995	A
5486359	Caplan et al.	Jan 1996	A
5494578	Brown et al.	Feb 1996	A
5494592	Latham, Jr. et al.	Feb 1996	A
5501371	Schwartz-Feldman	Mar 1996	A
5505685	Antwiler	Apr 1996	A
5510102	Cochrum	Apr 1996	A
5520885	Coelho et al.	May 1996	A
5525477	Hassouna	Jun 1996	A
5533518	Vogler	Jul 1996	A
5560830	Coleman et al.	Oct 1996	A
5575778	Hardt et al.	Nov 1996	A
5577513	Van Vlasselaer	Nov 1996	A
5585007	Antanavich et al.	Dec 1996	A
5588958	Cunningham et al.	Dec 1996	A
5589462	Patat et al.	Dec 1996	A
5601727	Bormann et al.	Feb 1997	A
5603845	Holm	Feb 1997	A
5607579	Latham, Jr. et al.	Mar 1997	A
5614106	Payrat et al.	Mar 1997	A
5618663	Delmas et al.	Apr 1997	A
5632895	Tsukagoshi et al.	May 1997	A
5632905	Haynes	May 1997	A
5641414	Brown	Jun 1997	A
5641622	Lake et al.	Jun 1997	A
5643192	Hirsh et al.	Jul 1997	A
5645540	Henniges et al.	Jul 1997	A
5646004	Van Vlasselaer	Jul 1997	A
5648223	Van Vlasselaer	Jul 1997	A
5649903	Deniega et al.	Jul 1997	A
5663051	Vlasselaer	Sep 1997	A
5674173	Hlavinka et al.	Oct 1997	A
5707331	Wells et al.	Jan 1998	A
5707647	Dunn et al.	Jan 1998	A
5707876	Levine	Jan 1998	A
5716616	Prockop et al.	Feb 1998	A
5723331	Tubo et al.	Mar 1998	A
5724988	Dennehey et al.	Mar 1998	A
5733466	Benebo et al.	Mar 1998	A
5733545	Hood, III	Mar 1998	A
5736033	Coleman et al.	Apr 1998	A
5738784	Holm et al.	Apr 1998	A
5738796	Bormann et al.	Apr 1998	A
5750025	Holmes et al.	May 1998	A
5750658	Coelho et al.	May 1998	A
5762798	Wenthold et al.	Jun 1998	A
5785700	Olson	Jul 1998	A
5786217	Tubo et al.	Jul 1998	A
5788662	Antanavich et al.	Aug 1998	A
5792344	Holm	Aug 1998	A
5795489	Holm	Aug 1998	A
5795571	Cederholm-Williams et al.	Aug 1998	A
5795751	Apel	Aug 1998	A
5811094	Caplan et al.	Sep 1998	A
5811151	Hendriks et al.	Sep 1998	A
5817519	Zelmanovic et al.	Oct 1998	A
5823986	Peterson	Oct 1998	A
5824084	Muschler	Oct 1998	A
5830359	Knight et al.	Nov 1998	A
5833866	Brown	Nov 1998	A
5834418	Brazeau et al.	Nov 1998	A
5837150	Langley et al.	Nov 1998	A
5840502	Van Vlasselaer	Nov 1998	A
5860937	Cohen	Jan 1999	A
5863892	Stern et al.	Jan 1999	A
5865785	Bischof	Feb 1999	A
5885239	Headley et al.	Mar 1999	A
5889584	Wardlaw	Mar 1999	A
5895346	Wells et al.	Apr 1999	A
5899874	Jonsson et al.	May 1999	A
5900245	Sawhney et al.	May 1999	A
5906934	Grande et al.	May 1999	A
5916557	Berlowitz-Tarrant et al.	Jun 1999	A
5916743	Lake et al.	Jun 1999	A
5918622	Perez et al.	Jul 1999	A
5924972	Turvaville et al.	Jul 1999	A
5934803	Hutter	Aug 1999	A
5938621	Kelly et al.	Aug 1999	A
5955032	Kelly et al.	Sep 1999	A
5955436	Kunkle, Jr.	Sep 1999	A
5958250	Brown et al.	Sep 1999	A
5958253	Holm et al.	Sep 1999	A
5980734	Itoh et al.	Nov 1999	A
5985315	Patat et al.	Nov 1999	A
6007811	Sawyer et al.	Dec 1999	A
6010627	Hood, III	Jan 2000	A
6020196	Hu et al.	Feb 2000	A
6022306	Dumont et al.	Feb 2000	A
6025201	Zelmanovic et al.	Feb 2000	A
6027655	Holm	Feb 2000	A
6049026	Muschler	Apr 2000	A
6051146	Green et al.	Apr 2000	A
6051147	Bischof	Apr 2000	A
6053856	Hlavinka	Apr 2000	A
6054122	MacPhee et al.	Apr 2000	A
6063297	Antanavich et al.	May 2000	A
6063624	Kandler et al.	May 2000	A
6071421	Brown	Jun 2000	A
6071422	Hlavinka et al.	Jun 2000	A
6071423	Brown et al.	Jun 2000	A
6090793	Zimmermann et al.	Jul 2000	A
6096309	Prior et al.	Aug 2000	A
6117425	MacPhee et al.	Sep 2000	A
6123655	Fell et al.	Sep 2000	A
6150163	McPherson et al.	Nov 2000	A
6153113	Goodrich et al.	Nov 2000	A
6183737	Zaleske et al.	Feb 2001	B1
6196987	Holmes et al.	Mar 2001	B1
6197325	MacPhee et al.	Mar 2001	B1
6200287	Keller et al.	Mar 2001	B1
6200606	Peterson et al.	Mar 2001	B1
6214338	Antanavich et al.	Apr 2001	B1
6221315	Giesler et al.	Apr 2001	B1
6245900	Yamasaki et al.	Jun 2001	B1
6264890	Boehringer et al.	Jul 2001	B1
6274090	Coelho et al.	Aug 2001	B1
6277961	Hock et al.	Aug 2001	B1
6280400	Niermann	Aug 2001	B1
6296602	Headley	Oct 2001	B1
6316247	Katz et al.	Nov 2001	B1
6322785	Landesberg et al.	Nov 2001	B1
6327491	Franklin et al.	Dec 2001	B1
6328765	Hardwick et al.	Dec 2001	B1
6342157	Hood, III	Jan 2002	B1
6351659	Vilsmeier	Feb 2002	B1
6355239	Bruder et al.	Mar 2002	B1
6368298	Beretta et al.	Apr 2002	B1
6368498	Guilmette	Apr 2002	B1
6398972	Blasetti et al.	Jun 2002	B1
6406671	DiCesare et al.	Jun 2002	B1
6410344	Chung et al.	Jun 2002	B1
6417004	Brady et al.	Jul 2002	B1
6440444	Boyce et al.	Aug 2002	B2
6444228	Baugh et al.	Sep 2002	B1
6464624	Pages	Oct 2002	B2
6471069	Lin et al.	Oct 2002	B2
6472162	Coelho et al.	Oct 2002	B1
6508778	Verkaart et al.	Jan 2003	B1
6516953	DiCesare et al.	Feb 2003	B1
6523698	Dennehey et al.	Feb 2003	B1
6544162	Van Wie et al.	Apr 2003	B1
6544727	Hei	Apr 2003	B1
6558341	Swisher	May 2003	B1
6596180	Baugh et al.	Jul 2003	B2
6623959	Harris	Sep 2003	B2
6629919	Egozy et al.	Oct 2003	B2
6638503	Chitte et al.	Oct 2003	B2
6676629	Andrew et al.	Jan 2004	B2
6719901	Dolecek et al.	Apr 2004	B2
6733471	Ericson et al.	May 2004	B1
6758978	Bedell	Jul 2004	B1
6777231	Katz et al.	Aug 2004	B1
6803022	DiCesare et al.	Oct 2004	B2
6811777	Mishra	Nov 2004	B2
6830762	Baugh et al.	Dec 2004	B2
6835353	Smith et al.	Dec 2004	B2
6835377	Goldberg et al.	Dec 2004	B2
RE38730	Wells et al.	Apr 2005	E
6899813	Dolecek et al.	May 2005	B2
6905612	Dorian et al.	Jun 2005	B2
6911202	Amir et al.	Jun 2005	B2
RE38757	Wells et al.	Jul 2005	E
7011644	Andrew et al.	Mar 2006	B1
7077273	Ellsworth et al.	Jul 2006	B2
7077827	Greenfield	Jul 2006	B2
7155288	Soykan et al.	Dec 2006	B2
7179391	Leach et al.	Feb 2007	B2
7195606	Ballin	Mar 2007	B2
7223346	Dorian et al.	May 2007	B2
7273886	Olivero et al.	Sep 2007	B2
7354515	Coull et al.	Apr 2008	B2
7374678	Leach et al.	May 2008	B2
7411006	Shanbrom	Aug 2008	B2
7470371	Dorian et al.	Dec 2008	B2
7531355	Rodriguez et al.	May 2009	B2
7553413	Dorian et al.	Jun 2009	B2
7845499	Higgins et al.	Dec 2010	B2
7914689	Higgins et al.	Mar 2011	B2
8048321	Leach et al.	Nov 2011	B2
8062534	Higgins et al.	Nov 2011	B2
20010009757	Bischof et al.	Jul 2001	A1
20020035820	Farris	Mar 2002	A1
20020076400	Katz et al.	Jun 2002	A1
20020082220	Hoemann et al.	Jun 2002	A1
20020090711	Karlsson	Jul 2002	A1
20020104808	Blasetti et al.	Aug 2002	A1
20020114775	Pathak	Aug 2002	A1
20020161449	Muschler	Oct 2002	A1
20020169408	Beretta et al.	Nov 2002	A1
20020172666	Sacchi et al.	Nov 2002	A1
20020182664	Dolecek et al.	Dec 2002	A1
20020192632	Hei et al.	Dec 2002	A1
20030033021	Plouhar et al.	Feb 2003	A1
20030033022	Plouhar et al.	Feb 2003	A1
20030050709	Noth et al.	Mar 2003	A1
20030050710	Petersen et al.	Mar 2003	A1
20030082152	Hedrick et al.	May 2003	A1
20030185803	Kadiyala et al.	Oct 2003	A1
20030191429	Andrew et al.	Oct 2003	A1
20030205538	Dorian et al.	Nov 2003	A1
20040013575	Stevens et al.	Jan 2004	A1
20040120942	McGinnis et al.	Jun 2004	A1
20040171146	Katz et al.	Sep 2004	A1
20040182395	Brookman	Sep 2004	A1
20040182788	Dorian et al.	Sep 2004	A1
20040182795	Dorian et al.	Sep 2004	A1
20040251217	Leach et al.	Dec 2004	A1
20050076396	Katz et al.	Apr 2005	A1
20050084961	Hedrick et al.	Apr 2005	A1
20050084962	Simon	Apr 2005	A1
20050109716	Leach et al.	May 2005	A1
20050130301	McKay et al.	Jun 2005	A1
20050153441	Hedrick et al.	Jul 2005	A1
20050153442	Katz et al.	Jul 2005	A1
20050186120	Dorian et al.	Aug 2005	A1
20050196393	Shanbrom	Sep 2005	A1
20050196874	Dorian et al.	Sep 2005	A1
20050247715	Ellsworth et al.	Nov 2005	A1
20050260174	Fraser et al.	Nov 2005	A1
20050260175	Hedrick et al.	Nov 2005	A1
20050282275	Katz et al.	Dec 2005	A1
20060051865	Higgins et al.	Mar 2006	A1
20060057693	Simon	Mar 2006	A1
20060083720	Fraser et al.	Apr 2006	A1
20060140923	Evangelista et al.	Jun 2006	A1
20060151384	Ellsworth et al.	Jul 2006	A1
20060175242	Dorian et al.	Aug 2006	A1
20060175244	Dorian et al.	Aug 2006	A1
20060178610	Nowakowski	Aug 2006	A1
20060196885	Leach et al.	Sep 2006	A1
20060243676	Swift et al.	Nov 2006	A1
20060273049	Leach et al.	Dec 2006	A1
20060273050	Higgins et al.	Dec 2006	A1
20060278588	Woodell-May	Dec 2006	A1
20070034579	Dorian et al.	Feb 2007	A1
20070036768	Fraser et al.	Feb 2007	A1
20070075016	Leach	Apr 2007	A1
20070208321	Leach et al.	Sep 2007	A1
20080011684	Dorian et al.	Jan 2008	A1
20080164204	Hatamian et al.	Jul 2008	A1
20080173593	Coull et al.	Jul 2008	A1
20080193424	McKale et al.	Aug 2008	A1
20080210645	Coull et al.	Sep 2008	A1
20080217263	Higgins et al.	Sep 2008	A1
20080217264	Leach et al.	Sep 2008	A1
20080217265	Leach et al.	Sep 2008	A1
20080268064	Woodell-May	Oct 2008	A1
20080269762	Simon et al.	Oct 2008	A1
20080283474	Leach et al.	Nov 2008	A1
20080306431	Yoo	Dec 2008	A1
20090014391	Leach et al.	Jan 2009	A1
20090018313	Shanbrom	Jan 2009	A1
20090101599	Dorian et al.	Apr 2009	A1
20090131827	Crocker et al.	May 2009	A1
20090192528	Higgins et al.	Jul 2009	A1
20090220482	Higgins et al.	Sep 2009	A1
20090221075	Dorian et al.	Sep 2009	A1
20090236297	Dorian et al.	Sep 2009	A1
20090250413	Hoeppner	Oct 2009	A1
20090253566	Chavarria	Oct 2009	A1
20100055087	Higgins et al.	Mar 2010	A1
20100140182	Chapman et al.	Jun 2010	A1
20100206798	Dorian et al.	Aug 2010	A1
20100256595	Leach et al.	Oct 2010	A1
20100323870	Leach et al.	Dec 2010	A1
20100324450	Leach et al.	Dec 2010	A1
20110014705	Leach et al.	Jan 2011	A1
20110020196	Grippi et al.	Jan 2011	A1
20110021334	Leach et al.	Jan 2011	A1
20110036786	Ellsworth	Feb 2011	A1
20110056893	Leach et al.	Mar 2011	A1
20110065183	Dorian et al.	Mar 2011	A1
20110077596	Higgins et al.	Mar 2011	A1
20110168193	Leach et al.	Jul 2011	A1
20110192804	Landrigan et al.	Aug 2011	A1
20120015796	Leach et al.	Jan 2012	A1

Foreign Referenced Citations (67)

Number	Date	Country
696278	Jan 1999	AU
9103724	Mar 1993	BR
1321138	Aug 1993	CA
2182862	Jun 1996	CA
2448415	Dec 2002	CA
1074709	Jul 1993	CN
56103	Oct 1860	DE
1443359	Nov 1968	DE
4202667	May 1993	DE
090997	Oct 1983	EP
0102773	Mar 1984	EP
0109374	May 1984	EP
0142339	May 1985	EP
0244834	Nov 1987	EP
0253198	Jan 1988	EP
0295771	Dec 1988	EP
0417818	Mar 1991	EP
534178	Mar 1993	EP
0534178	Mar 1993	EP
0592242	Apr 1994	EP
1005910	Jun 2000	EP
1006360	Jun 2000	EP
1289618	Mar 2003	EP
1406492	Apr 2004	EP
1427279	Jun 2004	EP
1467746	Oct 2004	EP
1509326	Mar 2005	EP
1670315	Jun 2006	EP
1716901	Nov 2006	EP
854715	Nov 1960	GB
60-053845	Mar 1985	JP
60250014	Dec 1985	JP
2036872	Feb 1990	JP
02071747	Mar 1990	JP
02129224	Oct 2000	JP
2004-305439	Nov 2004	JP
2005098704	Apr 2005	JP
2006-305365	Nov 2006	JP
WO-8400905	Mar 1984	WO
WO-8802259	Apr 1988	WO
WO-9010031	Sep 1990	WO
WO-9222312	Dec 1992	WO
WO-9305067	Mar 1993	WO
WO-9308904	May 1993	WO
WO-9407548	Apr 1994	WO
WO-9617871	Jun 1996	WO
WO-9617871	Jun 1996	WO
WO-9848938	Nov 1998	WO
WO-0061256	Oct 2000	WO
WO-0074713	Dec 2000	WO
WO-0103756	Jan 2001	WO
WO-0183068	Nov 2001	WO
WO-0238610	May 2002	WO
WO-02060925	Aug 2002	WO
WO-02098566	Dec 2002	WO
WO-03015800	Feb 2003	WO
WO-03024215	Mar 2003	WO
WO-03053362	Jul 2003	WO
WO-03088905	Oct 2003	WO
WO-03092894	Nov 2003	WO
WO-03099412	Dec 2003	WO
WO-2004009207	Jan 2004	WO
WO-2004104553	Dec 2004	WO
WO-2005034843	Apr 2005	WO
WO-2007127834	Nov 2007	WO
WO-2007142908	Dec 2007	WO
WO-2009021257	Feb 2009	WO

Non-Patent Literature Citations (150)

Entry
“Caps for Coming® and Costar® Plastic Labware,” Technical Bulletin. (Dec. 2008) Corning, Incorporated.
“Centrifuge Tubes” Corning Costar brochure. 1996/1997 Catalog pp. 76-77.
“Clotalyst® Autologous Clotting Factor” brochure. (Aug. 15, 2008) Biomet Biologics.
“Corning® 15 and 50 mL Centrifuge Tubes,” Life Sciences. (2005) Corning Incorporated.
“Letter CryoSeal FS System. Vaccines, Blood & Biologics,” letter. (Jul. 26, 2007) FDA U.S. Food and Drug Administation. http://www.fda.gov/BiologicsBloodVaccines/BloodBloodProducts/ApprovedProducts/Premarket ApprovalsPMAs/ucm091631.htm (Web accessed Aug. 12, 2011).
“Plasmax® Plasma Concentration System” brochure. (Jun. 15, 2008) Biomet® Biologics.
International Search Report and Written Opinon mailed Aug. 9, 2011 for PCT/US2011/031954 claiming benefit of U.S. Appl. No. 12/758,127, filed Apr. 12, 2010.
“Cell Isolation Techniques, Methods and Materials, Working with Enzymes,” (2004) (9 pages) Worthington Biochemical Corp.
“Cell Isolation Theory, Tissue Types,” (2004) (5 pages) Worthington Biochemical Corp.
“Clotalyst® Autologous Clotting Factor. Would you like to have an autologous thrombin for rapid clotting and haemostasis?” Brochure. Biomet Biologics (Aug. 15, 2008).
“Cytori Celution Cell Concentrate Device,” Exhibit 14, 510(k) Summary, FDA approval K060482 (Sep. 28, 2006).
“Frequently Asked Questions, 1. Kits, 2. Engzymes,” (2003) 3 pages Worthington Biochemical Corp.
“MarrowStim™ Concentration Kit Peripheral Arterial Disease (PAD) Study” brochure. Web. Jul. 2, 2009 http://www.biomet.com/patients/clinical—recruitment—padstudy.cfm.
“MarrowStim™ Concentration System,” brochure. Biomet Biologics Jun. 15, 2008.
“Prosys PRP Kit,” brochure Tozai Holdings, Inc. http://tozaiholdings.en.ec21.com/Prosys—PRP—Kit--5467051—5467061.html Printed from Web Aug. 24, 2011.
“Prosys PRP Kit,” Tozai Holdings, Inc. EC21 Global B2B Marketplace http://www.ec21.com/product-details/Prosys-PRP-Kit--5467061.html Printed from Web Jul. 18, 2011.
“ThermoGenesis Corp. to Supply Autologous Thrombin Kits to Biomet, Inc.,” PR Newslink: http:/tinyurl.com/4h3up. (Apr. 5, 2005) http://www.noblood.org/press-releases/2128-thermogenesis-corp-supply-autologous-thrombin-kits-biomet-inc [web accessed Sep. 27, 2011].
“Trypsinizing cells.” Bart's Cookbook, Web. Apr. 14, 2010. http://pingu.salk.edu/˜sefton/Hyper—protocols/trypsin.html.
Anesthesiology, vol. 81, No. 4, pp. 1074-1077, Oct. 1994, Hiromasa Mitsuhata, M.D., et al., “An Anaphylactic Reaction to Topical Fibrin Glue”.
Ann Thorac Surg, vol. 53, pp. 530-531, 1992, Mehmet C. Oz, M.D., et al., “Autologous Fibrin Glue From Intraoperatively Collected Platelet-Rich Plasma”.
Ann Thorac Surg, vol. 56, pp. 387-389, 1993, Robert L. Quigley, M.D., et al., “Intraoperative Procurement of Autologous Fibrin Glue”.
Badiavas, et al., “Treatment of Chronic Wounds With Bone Marrow-Derived Cells,” (Reprinted) Arch Dermatol. 139:510-516 (Apr. 2003).
Bang, N.U., et al., “Plasma Protein Requirements for Human Platelet Aggregation” Ann. N.Y. Acad Sci, 201:280-299 (1972).
Berguer, R., R. L. Staerkel, E. E. Moore, F. A. Moore, W. B. Galloway, and M. B. Mockus. “Warning: fatal reaction to the use of fibrin glue in deep hepatic wounds. Case reports.” J Trauma 31:3 (1991): 408-11.
Berruyer, M., J. Amiral, P. Ffrench, J. Belleville, O. Bastien, J. Clerc, A. Kassir, S. Estanove, and M. Dechavanne. “Immunization by bovine thrombin used with fibrin glue during cardiovascular operations. Development of thrombin and factor V inhibitors,” J Thorac Cardiovasc Surg 105: 5 (1993): 892-7.
BioCUE™ Platelet Concentration System, Dec. 2010. (2 pages).
Biopolymers, vol. 27, pp. 763-774, 1988, Gerald Marx, “Mechanism of Fibrin Coagulation Based on Selective, Cation-Driven, Protofibral Association”.
Boomgaard, et al., “Pooled Platelet Concentrates Prepared by the Platelet-Rich-Plasma Method and Filtered with Three Different Filters and Stored for 8 Days.” Vox Sang, vol. 68: 82-89, Feb. 1995.
Brodke, et al., “Bone Grafts Prepared with Selective Cell Retention Technology Heal Canine Segmental Defects as Effectively as Autograft”, SCR-Enriched Bone Crafts Heal Canine Segmental Defects, Journal of Orthopaedic Research (May 2006) pp. 857-866.
Casali, B., F. Rodeghiero, A. Tosetto, B. Palmieri, R. Immovilli, C. Ghedini, and P. Rivasi. “Fibrin glue from single-donation autologous plasmapheresis.” Transfusion 32:7 (1992): 641-3.
Clotalyst™, Automatic Clotting Factor, Would you like to have an autologous thrombin for rapid clotting and haemostasis?, brochure, Biomet Biologics, Inc., Feb. 2007 (12 pages).
Collier, B.S. et al., “The pH Dependence of Quantitative Ristocetin-induced Platelet Aggregation: Theoretical and Practical Implications—A New Device for Maintenance of Platelet-Rich Plasma pH”, Hematology Service, Clinical Pathology Department, Clinical Center, National Institutes of Health, Bethesda, Md. 20014, Blood, vol. 47, No. 5 (May 1976).
Connolly, “Injectable Bone Marrow Preparations to Stimulate Osteogenic Repair,” Clinical Orthopaedics and Related Research 313:8-18 (Apr. 1995).
Connolly, John, M.D., et al. “Development of an Osteogenic Bone-Marrow Preparation.” The Journal of Bone and Joint Surgery, Incorporated. vol. 71-A, No. 5 (Jun. 1989) pp. 684-691.
Dallari, et al., “In Vivo Study on the Healing of Bone Defects Treated with Bone Marrow Stromal Cells, Platelet-Rich Plasma, and Freeze-Dried Bone Allografts, Alone and in Combination,” Healing of Bone Defects, Journal of Orthopaedic Research (May 2006) pp. 877-888.
De Ugarte, et al., “Comparison of Multi-Lineage Cells from Human Adipose Tissue and Bone Marrow,” Cells Tissues Organs 174:101-109 (2003).
De Ugarte, et al., “Differential Expression of Stem Cell Mobilization-Associated Molecules on Multi-Lineage Cells from Adipose Tissue and Bone Marrow,” Immunology Letters 89:267-270 (2003).
DelRossi, A. J., A. C. Cernaianu, R. A.Vertrees, C. J. Wacker, S. J. Fuller, J. Cilley Jr., and W. A. Baldino. “Platelet-rich plasma reduces postoperative blood loss after cardiopulmonary bypass.” J Thorac Cardiovasc Surg 100:2 (Aug. 1990): 281-6.
DePalma, L., et al., “The preparation of fibrinogen concentrate for use as fibrin glue by four different methods.” Transfusion (1993) vol. 33, No. 9; pp. 717-720.
DeUgarte, M.D., Daniel A., et al., “Future of Fat as Raw Material for Tissue Regeneration,” (Feb. 2003) pp. 215-219, Lippincott Williams & Wilkins, Inc.
DiMuzio, Paul et al., “Development of a Tissue-Engineered Bypass Graft Seeded with Stem Cells,” Vasucular, vol. 14, No. 6, (2006) pp. 338-342, BC Decker, Inc.
Drug Intelligence and Clinical Pharmacy, vol. 22, pp. 946-952, Dec. 1988, Dennis F. Thompson, et al., “Fibrin Glue: A Review of Its Preparation, Efficacy, and Adverse Effects as a Topical Hemostat”.
Edlich, Richard F., George T. Rodeheaver, and John G. Thacker. “Surgical Devices in Wound Healing Management.” In Wound Healing: Biochemical & Clinical Aspects,ed. I. Kelman Cohen, Robert F. Diegelmann, and William J. Lindblad. 581-600. 1st ed., vol. Philadelphia: W.B. Saunders Company, 1992).
Eppley, et al., “Platelet Quantification and Growth Factor Analysis from Platelet-Rich Plasma: Implications for Wound Healing,” Plastic and Reconstructive Surgery, 114(6):1502-1508 (Nov. 2004).
Epstein, G. H., R. A. Weisman, S. Zwillenberg, and A. D. Schreiber. “A new autologous fibrinogen-based adhesive for otologic surgery.” Ann Otol Rhinol Laryngol 95 (May 25-26, 1985) 40-5.
Fibrostik™ Plasma Concentrator, Attention Operating Surgeon, Cell Factor Technologies, Inc., Jul. 2003.
First clinical results: Kuderma, H. and Helene Metres. “Die klinische Anwendung der Klebung van Nervenanastomosen mit Gerinnungssubstanzen bei der Rekonstruction verletzter peripherer Nerven.” Wein Klin Wochenschr 87 (Aug. 15, 1975): 495-501.
Floryan, K. et al. “Home Study Program: Intraoperative Use of Autologous Platelet-Rich and Platelet-Poor Plasma for Orthopedic Surgery Patients” vol. 80, No. 4 (Oct. 2004) p. 667-674.
Frasier, John K., et al., “Plasticity of human adipose stem cells toward endothelial cells and cardiomyocytes,” Nature Clinical Practice Cardiovascular Medicine, vol. 3, Supplement 1 (Mar. 2006) pp. S33-S37.
Friesen, M.D., Robert, et al. “Blood Conservation During Pediatric Cardiac Surgery: Ultrafiltration of the Extracorporeal Circuit Volume After Cardiopulmonary Bypass.” Anesth. Analg 1993: 77-702-7.
Galois, et al., “Cartilage Tissue Engineering: State-of-the-Art and Future Approaches,” Pathol Biol (Paris), 53(10), Dec. 2005.
Gibble, J. W. and P. M. Ness. “Fibrin glue: the perfect operative sealant?” Transfusion 30 (Aug. 1990): 741-7.
Gimble, Jeffrey M., “Adipose-Derived Stem Cells for Regenerative Medicine,” Circulation Research (May 11, 2007) pp. 1249-1260, American Heart Association, Inc.
Gomillion, Cheryl T., et al., “Stem cells and adipose tissue engineering,” Biomaterials 27, Science Direct (2006) pp. 6052-6063, Elsevier.
GPS® III System, GPS® III Platelet Separation System, Leadership through Technology, brochure, Jul. 2007 (8 sheets).
GPS® System, “GPS® Platelet Concentrate System,” Cell Factor Technologies, Inc., Biomet Orthopaedics, Inc., (Feb. 29, 2004) (9 pages).
GPS® System, “Shoulder Recovery with the GPS® Platelet Concentrate System, Rotator Cuff Surgical Techniques,” brochure, Cell Factor Technologies, Inc., Biomet Orthopaedics, Inc., (2004) 6 pages.
GPS® System, “Shoulder Recovery with the GPS® Platelet Concentrate System, Rotator Cuff Surgical Techniques,” Cell Factor Technologies, Inc., Biomet Orthopaedics, Inc., (2004) 3 pages, http://www.cellfactortech.com/global—products.cfm, printed Sep. 16, 2005.
GPS® II System, Gravitational Platelet Separation System, “Accelerating the Body's Natural Healing Process,” Biomet Biologics (Jul. 15, 2006) 16 pages.
GPS® II System, Gravitational Platelet Separation System, “Accelerating the Body's Natural Healing Process,” Cell Factor Technologies, Inc., Biomet Europe (2005) 16 pages, http://www.cellfactortech.com/global—products.cfm, printed Sep. 16, 2005.
GPS® II System, Gravitational Platelet Separation System, “User Manual,” Cell Factor Technologies, Inc., Biomet Europe [date unknown] 13 pages, http://www.cellfactortech.com/global—products.cfm, printed Sep. 16, 2005.
Grove, et al., “Plasticity of Bone Marrow-Derived Stem Cells,” Stem Cells: Concise Review, 22, Jan. 2004.
Guilak, Frank, et al., “Adipose-derived adult stem cells for cartilage tissue engineering,” Biorheology 41 (2004) pp. 389-399, IOS Press.
Harris, E.L.V. Concentration of the Extract. In. Protein Purification Methods: A Practical Approach Harris, E.L.V.; Angel, S.; Editors. (1989) Publisher: (IRL Press, Oxford, UK), pp. 67-69.
Hartman, A. R., D. K. Galanakis, M. P. Honig, F. C. Seifert, and C. E. Anagnostopoulos. “Autologous whole plasma fibrin gel. Intraoperative procurement.” Arch Surg 127 (Mar. 1992): 357-9.
Harvest SmartPrep PRP-20 Procedure Pack, “Instructions for Use” (date unknown).
Harvest Technologies brochure, SmartPrep2 (2002).
Hattori, et al., “Osteogenic Potential of Human Adipose Tissue-Derived Stromal Cells as an Alternative Stem Cell Source,” Cells Tissues Organs (2004) 178:2-12 Karger.
Haynesworth, S.E. et al. “Mitogenic Stimulation of Human Mesenchymal Stem Cells by Platelet Releasate Suggests a Mechanism for Enhancement of Bone Repair by Platelet Concentrate” 48th Annual Meeting of the Orthopaedic Research Society Poster No. 0462 (2002).
Hennis, H. L., W. C. Stewart, and E. K. Jeter. “Infectious disease risks of fibrin glue [letter].” Ophthalmic Surg 23 (Sep. 1992): 640.
Hernigou, et al., “Percutaneous Autologous Bone-Marrow Grafting for Nonunions. Influence of the Number and Concentration of Progenitor Cells,” Journal of Bone & Joint Surgery, 87-A(7):1430-1437 (Jul. 2005).
Hom, D., et al. “Promoting Healing with Recombinant Human Platelet-Derived Growth Factor-BB in a Previously Irradiated Problem Wound.” The Laryngoscope, vol. 113 (pp. 1566-1671) Sep. 2003.
Hood, Andrew G., et al., “Perioperative Autologous Sequestration III: A New Physiologic Glue with Wound Healing Properties,” (Jan. 1993) vol. 14 pp. 126-129.
International Preliminary Examination Report and Written Opinion issued Aug. 31, 2010 for PCT/US2009/035564 claiming benefit of U.S. Appl. No. 61/078,178, filed Jul. 3, 2008, which priority is also claimed of said provisional case by U.S. Appl. No. 12/395,085 filed Feb. 27, 2009.
International Preliminary Report on Patentability and Written Opinion mailed Oct. 13, 2011 for PCT/US2010/029957 which claims benefit of U.S. Appl. No. 12/417,789, filed Apr. 3, 2009.
International Preliminary Report on Patentability completed Aug. 13, 2009 for PCT/US2008/004687 claiming benefit of U.S. Appl. No. 60/911,407, filed Apr. 12, 2007.
International Preliminary Report on Patentability mailed Jan. 26, 2012 for PCT/US2010/041942 claiming benefit of U.S. Appl. No. 12/504,413, filed Jul. 16, 2009.
International Search Report and Written Opinion mailed Jul. 2, 2008 for International Application No. PCT/US2008/004687 which claims priority to U.S. Appl. No. 60/911,407, filed Apr. 12, 2007.
International Search Report and Written Opinion mailed Jul. 3, 2009 for PCT/US2009/035564 claiming benefit of U.S. Appl. No. 61/078,178, filed Jul. 3, 2008.
International Search Report and Written Opinion mailed Jul. 30, 2010 for PCT/US2010/029957 which claims benefit of U.S. Appl. No. 12/417,789, filed Apr. 3, 2009.
International Search Report and Written Opinion mailed Nov. 7, 2011 for PCT/US2011/045290 claiming benefit of U.S. Appl. No. 12/846,944, filed Jul. 30, 2010.
International Search Report and Written Opinion mailed Oct. 8, 2010 for PCT/US2010/041942 claiming benefit of U.S. Appl. No. 12/504,413, filed Jul. 16, 2009.
International Search Report for International Application No. PCT/US/0316506 mailed Oct. 13, 2003 which claims benefit of U.S. Appl. No. 60/383,013, filed May 24, 2002.
International Search Report for International Application No. PCT/US2007/012587 mailed Nov. 6, 2007 which claims benefit of U.S. Appl. No. 11/441,276, filed May 25, 2006.
Ishida, et al., “Platelet-Rich Plasma With Biodegradable Gelatin Hydrogel Promotes Rabbit Meniscal Tissue Regeneration,” 52nd Annual Meeting of the Orthopaedic Research Society Paper No. 1035, 1 page (2006).
Jackson, C. M. and Y. Nemerson. “Blood coagulation.” Annu Rev Biochem 49 (Aug. 11, 1980):765-811).
Jayadev, Suprya. “Trypsinization of Adherent Cells.” Aug. 8, 1991. Web. Apr. 14, 2010 http://www.duke.edu/web/ceramide/protocols/0005.html.
Johnstone, et al., “Autologous Mesenchymal Progenitor Cells in Articular Cartilage Repair”, Clinical Orthopaedics and Related Research 367S:S156-S162 (Oct. 1999).
Jorgensen, et al., “Stem Cells for Repair of Cartilage and Bone: The Next Challenge in Osteoarthritis and Rheumatoid Arthritis,” Annals of Rheumatic Diseases, Aug. 2000.
Journal of Oral Maxillofacial Surgery, vol. 43, pp. 605-611, Helene Matras, M.D., “Fibrin Seal: The State of the Art” (1985).
Karpatkin, S., “Heterogeneity of Human Platelets. VI., Correlation of Platelet Function with Platelet Volume”, Blood, vol. 51, No. 2 (Feb. 1978).
Kjaergard, H. K,, U. S. Weis-Fogh, H. Sorensen, J. Thiis, and I. Rygg. “A simple method of preparation o£ autologous fibrin glue by means of ethanol.” Surg Gynecol Obstet 175 (Jan. 1992): 72-3.
Kjaergard, H. K., Fogh Us Weis, and J. J. ThHs. “Preparation of autologous fibrin glue from pericardial blood.” Ann Thorac Sur 55 (Feb. 1993): 543-4.
Kumar, Vijay et al. “Stability of Human Thrombin Produced From 11 ml of Plasma Using the Thrombin Processing Device,” Journal of American Society of Extra-Corporeal Technology. JECT: Mar. 2005:37; 390-395.
Kumar, Vijay et al. “Whole Blood Thrombin: Development of a Process for Intra-Operative Production of Human Thrombin.” Journal of American Society of Extra-Corporeal Technology. JECT: Apr. 2007; 39:18-23.
Kumar, Vijay et al., “Autologous Thrombin: Intraoperative Production From Whole Blood.” Journal of American Society of Extra-Corporeal Technology. JECT: Apr. 2008; 40:94-98.
Laryngoscope vol. 99, pp. 974-976, Sep. 1989, Kyosti Laitakari, M.D., et al., “Autologous and Homologous Fibrinogen Sealants: Adhesive Strength”.
Laryngoscope, vol. 95, pp. 1074-1076, Sep. 1985, Karl H. Siedentop, M.D., et al., “Autologous Fibrin Tissue Adhesive”.
Laryngoscope, vol. 96, pp. 1062-1064, Oct. 1986, Karl H. Siedentop, M.D., et al., “Extended Experimental and Preliminary Surgical Findings with Autologous Fibrin Tissue Adhesive Made from Patient's Own Blood”.
Lasher, Lisa, M.D., “My Experience with PRP,” PowerPoint presentation, http://www.cellfactortech.com/global—products.cfm, printed Sep. 16, 2005.
Lendeckel, Stefan, et al., “Autologous stem cells (adipose) and fibrin glue used to treat widespread traumatic calvarial defects: case report,” Journal of Cranio-Maxillofacial Surgery (2004) European Association for Cranio-Maxillofacial Surgery.
Lerner, R. and N. S. Binur. “Current status of surgical adhesives.” J Surg Res 48 (Feb. 1990): 165-81.
Longas, Maria O., “An Improved Method for the Purification of Human Fibrinogen.” J. Biochem (1980) vol. 11, pp. 559-564.
Lu, et al., “Bone Marrow Mesenchymal Stem Cells: Progress in Bone/Cartilage Defect Repair,” 19(1), Jan. 2002.
Marrowstim Concentration System, Biomet Biologics, Inc., 20 pages (REV Feb. 15, 2008).
Marx, Gerard, et al., “Heat Denaturation of Fibrinogen to Develop a Biomedical Matrix.” Journal of Biomedical Materials Research Part B: Applied Biomaterials (Apr. 2007) pp. 49-57.
Masri, Marwan A., et al. “Isolation of Human Fibrinogen of High Purity and in High Yield Using Polyethylene Glycol 1000.” Thromb Haemostas (Stuttgart) (1983) vol. 49 (2); pp. 116-119.
Matras, Helene, H. P. Dinges, H. Lassmann, and B. Mamoli. “Zur nahtlosen interfaszikularen Nerventransplantation im Tierexperiment.” Wein Med Woschtr 122:37 (1972): 517-523.
Minntech® Filtration Technologies Group, “Hemocor HPH® Hemoconcentrator,” Minntech Corporation (2004); http://www.minntech.com/ftg/products/hph/index.html, printed Jul. 15, 2004 (2 pages).
Minntech® Filtration Technologies Group, “Medical Applications: Blood Filtration” Minntech Corporation (2004); http://www.minntech.com/ftg/industries/medical/blood—filter.html, printed Jul. 15, 2004 (1 page).
Minntech® Filtration Technologies Group, “Renaflo® II Hemofilter,” Minntech Corporation (2004); http://www.minntech.com/ftg/products/renaflo/index.html, printed Jul. 15, 2004 (2 pages).
Molnar, Amy, “Stem Cells from Muscles Can Repair Cartilage, Study Finds Genetically Engineered Muscle-Derived Stem Cells Improved Cartilage Repair in Rats”, American College of Rheumatology, (2005).
Moretz, W., Jr., J Shea Jr., J. R. Emmett, and J Shea. “A simple autologous fibrinogen glue for otologic surgery.” Otolaryngol Head Neck Surg 95 (Jul. 1986): 122-4.
Nakagami, Hironori, et al., “Novel Autologous Cell Tehrapy in Ischemic Limb Disease Through Growth Factor Secretion by Cultured Adipose Tissue-Derived Stromal Cells,” Angiogenesis by Adipose Tissue-Derived Cells, (Dec. 2005) pp. 2542-2547, American Heart Association, Inc.
Nathan, Suresh,, et al., “Cell-Based Therapy in the Repair of Osteochondral Defects: A Novel Use for Adipose Tissue,” Tissue Engineering, vol. 9, No. 4 (2003) pp. 733-744 Mary Ann Liebert, Inc.
Nilsson, et al., “Bone Repair Induced by Bone Morphogenetic Protein in Ulnar Defects in Dogs,” The Journal of Bone and Joint Surgery, vol. 68 B., No. 4, Aug. 1986.
Orphardt, Charles E., “Denaturation of Proteins,” Virtual Chembook, Elmhurst College (2003) 3 pages. http://www.elmhurst.edu/˜chm/vchembook/568denaturation.html (web accessed Mar. 9, 2011).
Otolaryngologic Clinics of North America, vol. 27, No. 1, pp. 203-209, Feb. 1994, Dean M. Toriumi, M.D., et al., “Surgical Tissue Adhesives in Otolaryngology-Head and Neck Surgery”.
Parker, Anna M., et al., Adipose-derived stem cells for the regeneration of damaged tissues, Expert Opinion, Cell- & Tissue-based Therapy, Expert Opin. Biol. Ther. (2006) pp. 567-578 Informa UK Ltd.
Planat-Bénard, V., et al., “Spontaneous Cardiomyocyte Differentiation From Adipose Tissue Stroma Cells,” Adipose-Derived Cell Cardiomyocyte (Feb. 6, 2004) pp. 223-229 American Heart Association, Inc.
Ponticiello, Michael S., “A Rapid Technique for the Isolation and Concentration of Stem Cells from Human Bone Marrow”, Cell Factor Technologies, Inc. (2006) 2 pages.
Rangappa, Sunil, M.D., “Transformation of Adult Mesenchymal Stem Cells Isolated From the Fatty Tissue Into Cardiomyocytes,” Adult Stem Cells Transformed into Cardiomyoctyes, (2003) pp. 775-779 Ann Thorac Surg.
Rigotti, M.D., et al, “Clinical Treatment of Radiotherapy Tissue Damage by Lipoaspirate Transplant: a Healing Process Mediated by Adipose-Derived Adult Stem Cells,” Plastic and Reconstructive Surgery, Breast, PRS Journal vol. 119, No. 5, Stem Cell Therapy for Angiogenesis, (Apr. 15, 2007) pp. 1409-1422.
Rubin, M.D., et al, “Clinical Treatment of Radiotherapy Tissue Damage by Lipoaspirate Transplant: A Healing Process Mediated by Adipose-Derived Adult Stem Cells,” Plastic and Reconstructive Surgery, Discussion vol. 119, No. 5, Stem Cell Therapy for Angiogenesis, (Apr. 15, 2007) pp. 1423-1424.
Sanal, M. “Does fibrin glue cause foreign body reactions? [letter].” Eur J Pediatr Surg 3 (1992): 190 (1 page).
Sanal, M., H. Dogruyol, A. Gurpinar, and O. Yerci. “Does fibrin glue cause foreign body reactions?” Eu r J Pediatr Surg 2 (1992): 285-6.
Schmidt, K.G., et al., “Labelling of Human and Rabbit Platelets with Indium-Oxine Complex”, 23:97-106 (1979).
Schmidt, K.G., et al., “Preparation of Platelet Suspensions from Whole Blood in Buffer”, Scand. J. Hoemato, 23:88-96 (1979).
Schäffler, Andreas, et al., “Concise Review: Adipose Tissue-Derived Stromal Cells—Basic and Clinical Implications for Novel Cell-Based Therapies,” Tissue-Specific Stem Cells, Stem Cells® (Apr. 10, 2007) pp. 818-827 AlphaMed Press.
Semple, Elizabeth, PhD, et al. “Quality of Thrombin Produced From the Patient's Own Plasma Using the TPD Tradmark in Here, a New Thrombin-Processing Device.” Journal of American Society of Extra-Corporeal Technology. JECT: 2005; 37:196-200.
Sierra, D. H. “Fibrin sealant adhesive systems: a review of their chemistry, material properties and clinical applications.” J Biomater Appl 7 (Apr. 1993): 309-52.
Sigma-Aldrich® Alkaline Phosphatase (Procedure No. 85), drug fact sheet, (2003) pp. 1-2, Sigma-Aldrich, Inc.
Silver, Frederick H., et al., “Review Preparation and use of fibrin glue in surgery.” Biomaterials 16 (1995) pp. 891-903.
Solem, Jan Otto, et al., “Hemoconcentration by Ultrafiltration During Open-Heart Surgery,” Scand J Thor Cardiovasc Surg 22:271-274, 1988.
Sutton, Robin G., et al. “Comparison of Three Blood-Processing Techniques During and After Cardiopulmonary Bypass.” Ann Thorac Surg (1993) vol. 56; pp. 941-943.
Swift, Mathew J., et al., “Characterization of Growth Factors in Platelet Rich Plasma,” 1-Cell Factor Technologies, http://www.cellfactortech.com/global—products.cfm, printed Sep. 16, 2005.
Symphony II Platelet Concentrate System/PCS brochure; “Increasing bone graft bioactivity through reproducible concentrations of natural growth factors,” DePuy (Jan. 2003).
Takahashi, Kazutoshi et al., “Induction of Pluripotent Stem Cells from Adult Human Fibroblasts by Defined Factors,” Cell, (Nov. 30, 2007) pp. 1-12, Elsevier Inc.
The American Journal of Surgery, vol. 168, pp. 120-122, Aug. 1994, Roy L. Tawes, Jr., M.D., et al., “Autologous Fibrin Glue: The Last Step in Operative Hemostatis”.
The American Surgeon, vol. 55, pp. 166-168, Mar. 1989, William D. Spotnitz, M.D., et al., “Successful Use of Fibrin Glue During 2 Years of Surgery at a University Medical Center”.
The Sports Medicine Center, “Knee Cartilage Implantation”, Carticel™, “Autologous Cultured Chondrocyte Implantation”, http://www.orthoassociates.com/carticel.htm (printed Apr. 6, 2006).
The Stone Clinic, “Platelet Rich Plasma (PRP)”, web site printed May 2006.
Weis-Fogh, U. S. “Fibrinogen prepared from small blood samples for autologous use in a tissue adhesive system.” Eur Surg Res 20 (1988): 381-9.
Weisman, MD., Robert A., “Biochemical Characterization of Autologous Fibrinogen Adhesive,” Laryngoscope 97: Oct. 1987; pp. 1186-1190.
Wiseman, David M., David T. Rovee, and Oscar M. Alverez. “Wound Dressings: Design and Use.” In Wound Healing: Biochemical & Clinical Aspects,ed. I. Kelman Cohen, Robert F. Diegelmann, and William J. Lindblad. 562-580. 1st ed., vol. Philadelphia: W. B. Saunders Company, 1992.
Woodell-May, et al., “Producing Accurate Platelet Counts for Platelet Rich Plasma: Validation of a Hematology Analyzer and Preparation Techniques for Counting,” Scientific Foundation, Journal of Camiofacial Surgery 16(5):749-756 (Sep. 2005).
Written Opinion of the International Preliminary Examining Authority mailed Mar. 17, 2009 for International Application No. PCT/US2008/004687 which claims priority to U.S. Appl. No. 60/911,407, filed Apr. 12, 2007.
Yoon, Eulsik, M.D., Ph.D., et al., “In Vivo Osteogenic Potential of Human Adipose-Derived Stem Cells/Poly Lactide-Co-Glycolic Acid Constructs for Bone Regneration in a Rat Critical-Sized Calvarial Defect Model,” Tissue Engineering, vol. 13, No. 3 (2007) pp. 619-627 Mary Ann Liebert, Inc.
Zhang, Duan-zhen, et al., “Transplantation of autologous adipose-derived stem cells ameliorates cardiac function in rabbits with myocardial infarction,” Chinese Medical Journal, vol. 120, No. 4 (2007) pp. 300-307 General Hospital of Shenyang Military Region, Shenyang, China.
Zuk, Patricia A., Ph.D., “Multilineage Cells from Human Adipose Tissue: Implications for Cell-Based Therapies,” Tissue Engineering, vol. 7, No. 2, (2001) pp. 211-228 Mary Ann Liebert, Inc.

Related Publications (1)

	Number	Date	Country
	20110251041 A1	Oct 2011	US

Method and apparatus for separating a material

Information

Patent Number

Date Filed

Date Issued

Inventors

Original Assignees

Examiners

Agents

CPC

US Classifications

Field of Search

US

International Classifications