Patent Grant
9550028
This section provides background information related to the present disclosure which is not necessarily prior art.
Biological materials are routinely processed in order to enhance various properties or characteristics of the biological materials. For example, whole blood is often harvested from a patient or retrieved from a blood bank, and fractionated. The whole blood can be fractionated into a red blood cell concentrate, platelet-rich plasma, platelet-poor plasma, or an autologous protein solution. Likewise, bone marrow aspirate is often harvested and processed to generated concentrated bone marrow aspirate. The type of biological material being processed and the type of processing to be performed depend on individual patients and the conditions being treated.
Although biological materials are routinely processed, the devices used to process the materials are usually complex, costly, and require elaborate processing schemes. Such devices are often bulky and the processing schemes typically require multiple processing steps, which typically include centrifugations. Often, multiple centrifugation steps are necessary in order for a medical practitioner to arrive at the desired product. The centrifugation steps are timely and can result in product loss when isolating fractions.
Therefore, there is currently a need for new devices for processing biological materials that are cost effective, easy to use, and that require fewer processing steps than currently available devices.
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 technology provides a device for processing a biological material. The device comprises a syringe barrel having an inner diameter about a longitudinal axis, an open end, a closed end, and an outlet at the closed end. Desiccating beads are positioned within the barrel. The device further comprises a filter positioned at the closed end of the barrel, a plunger comprising a paddle assembly insertable into the barrel though the open end, and a needle. The filter comprises pores with diameters smaller than a diameter of the beads, but larger than a diameter of the biological material. The paddle assembly is configured to mix the biological material with the desiccating beads.
The present technology also provides for a device for processing a biological material comprising a syringe barrel having an inner diameter about a longitudinal axis from an open end to a closed end, and having an outlet at the closed end, wherein polyacrylamide beads are positioned within the barrel. A filter positioned at the closed end of the barrel, wherein the filter allows biological materials to pass through, but not the polyacrylamide beads. The device also has a plunger insertable into the barrel through the open end, the plunger having a paddle assembly, wherein the paddle assembly comprises a stem that extends along the longitudinal axis of the barrel and a plurality of paddles that extend radially from the stem. The device also has a needle. The device is configured to aspirate a biological material from a patient, process the biological material, and return the processed biological material back to the patient.
The present technology additionally provides for a method for processing a biological material. The method comprises aspirating a biological material from a patient, through a filter, and into a syringe assembly, the syringe assembly having a needle, a barrel, the filter, and a plunger, wherein a plurality of beads are positioned within the barrel, and wherein the plunger comprises a paddle assembly. The method further comprises turning a knob on the plunger, whereby the paddle assembly turns to mix the beads with the biological material to yield a processed biological material.
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.
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.
Corresponding reference numerals indicate corresponding parts throughout the several views of the drawings.
Example embodiments will now be described more fully with reference to the accompanying drawings
The present technology generally provides devices and methods for processing a biological material. The device draws a biological material from a patient, and processes the biological material. The processed biological material is then administered to the patient or combined with a graft material or implant. The patient can be a human or a non-human mammal, such as a dog, cat, or horse. Accordingly, methods include processing a biological material from a patient in a device according to the current disclosure to generate a processed biological material, and administering the processed biological material to the patient.
The devices comprise beads, which are used to process biological material. The beads can comprise any suitable material for processing the biological material. The beads can be a material comprising various polymers, metals, ceramics, or glasses. In some embodiments, the beads comprise a hygroscopic material. Examples of suitable materials include glasses, minerals, polymers, metals, and polysaccharides. Minerals include corundum and quartz. Polymers include polystyrene, polyethylene, polyvinyl chloride, polypropylene, and polyacrylamide. Metals include titanium. Polysaccharides include dextran and agarose. A preferred material comprises, or consists essentially of, polyacrylamide. Preferably, the beads comprise a desiccating material. In various embodiments, the beads are conjugated with an activating material, such as an antibody. Immunoglobulin g is a non-limiting example of such an antibody.
The beads can concentrate the biological material, induce a phenotypic change in the biological material, or both. Therefore, the size and composition of the beads can be altered based on the biological material to be processed and the application. Non-limiting examples of biological material include whole blood, bone marrow, adipose tissue, and chondrocytes. The biological material is processed in the device to generate processed biological materials, such as concentrated blood, platelet-poor plasma, platelet-rich plasma, autologous protein solution, concentrated bone marrow, concentrated adipose tissue, concentrated chondrocytes, and M2 macrophages. For example, when macrophages in whole blood contact polyacrylamide beads, the polyacrylamide beads induce the macrophages to polarize into the M2 phenotype.
Devices according to the current technology can be used for a variety of applications. For example, the devices can be used in the treatment of inflammation, osteoarthritis, microfractures, meniscus implants, meniscus transplants, or other orthopedic implants or transplants. Uses further include treating osteolysis resulting from wear debris and inflammation at the site of an artificial joint in a patient. The device can be used for a laparoscopic preparation of, for example, an autologous protein solution, concentrated bone marrow aspirate, or platelet-rich plasma.
With reference to
The device further comprises a filter 28 that comprises pores with diameters smaller than a diameter of the beads 26, but larger than a diameter of the biological material. The filter 28 can be positioned within the barrel 12, at the closed end 20.
The device 10 further comprises a plunger 30 that is partially inserted into the barrel 12 through the open end 18. Accordingly, the plunger 30 has an exterior portion 32 and an interior portion 34. The plunger 30 has a diameter substantially similar to the inner diameter 14 of the barrel 12. The exterior portion 32 of the plunger 30 comprises a knob 36. The interior portion 34 of the plunger 30 has an end 38, which is coupled to a paddle assembly 40. As shown in
The device 10 is used to withdraw biological material from a patient by inserting the needle 24 into the patient and drawing back on the plunger 30. The biological material is then processed by incubating the biological material with the beads 26 and turning knob 36 to mix the biological material and the beads 26 with the paddle assembly 40. The processed biological material can then be administered to the patient by utilizing the needle 24 or replacing the needle 24 with a new, sterile needle, inserting the needle 24 or new needle into the patient, and depressing the plunger 30 until a desired volume of the processed biological material has been administered into the patient. Depressing the plunger 30 causes the paddle assembly 40 to become compressed between the end 38 of the plunger 30 and the filter 28. This results in the paddle assembly 40 collapsing or breaking so that the plunger 30 can be depressed further. Alternatively, the processed biological material is combined with a graft material or with an implant.
The device 50 further comprises a plunger 66 that is partially inserted into the barrel 52 through the open end 58. Accordingly, the plunger 66 has an exterior portion 68 and an interior portion 70. The plunger 66 has a diameter substantially similar to the inner diameter 54 of the barrel 52. The exterior portion 68 of the plunger 66 comprises a knob 72. The interior portion 70 of the plunger 66 has an end 74, which is coupled to a paddle assembly 76. As shown in
The device 50 further comprises a removable filter 82 comprising a syringe-coupling port 84 and a needle-coupling port 86 opposite the syringe-coupling port. The syringe-coupling port 84 couples the filter 82 to the barrel 52 and the needle-coupling port 86 couples the filter 82 to a needle 88. The filter 82 comprises pores that are smaller than a diameter of the beads 64, but larger than a diameter of the biological material to be processed. Therefore, the filter 82 can be selectively chosen from a plurality of filters with differing pore sizes based on the size of the biological material to be processed as long as the pore size is smaller than the diameter of the beads 64. For example, various filters can exclude platelets, leukocytes, or red blood cells from whole blood. The device 50 is used to withdraw a biological material from a patient, process the biological material, and either to administer the processed biological material to the patient or to combine the processed biological material with a graft material or implant.
The device 90 further comprises a filter 108 that comprises pores with diameters smaller than a diameter of the beads 106, but larger than a diameter of the biological material. The filter 108 can be positioned within the barrel 92, at the closed end 100.
The device 90 further comprises a plunger 110 that is partially inserted into the barrel 92 through the open end 98. Accordingly, the plunger 110 has an exterior portion 112 and an interior portion 114. The plunger 110 has a diameter substantially similar to the inner diameter 94 of the barrel 92. The exterior portion 112 of the plunger 110 comprises a knob 116. The interior portion 114 of the plunger 110 has an end 118, which is coupled to a paddle assembly 120. As shown in
As shown in
After processing, the cap 128 is removed and a new needle 130 can be attached to the outlet 102, as in
The present technology also provides methods for processing a biological material, which can be performed at a point of care. The present technology provides methods where the processing of a biological material is performed at a time proximate to administration of the processed biological material. For example, such proximate administration of the processed biological material may be performed 1 hour, 30 minutes, 15 minutes, 10 minutes, 2 minutes, 1 minute, or less, after harvesting the biological material from a patient. In some processes, the methods are “point of care,” wherein the processes of the present technology are performed at a location proximate, such as in the same room (for example, bed side) or otherwise immediately adjacent, to the mammalian subject undergoing treatment. The methods enable laparoscopic preparation of, for example, an autologous protein solution, concentrated bone marrow aspirate, or platelet-rich plasma. In an embodiment, the biological material is autologous to the patient to whom it will be administered
The device 10 of
As shown in
In
The method can be performed in the treatment of inflammation, osteoarthritis, microfractures, meniscus implants, meniscus transplants, or other orthopedic implants or transplants. Uses further include treating osteolysis resulting from wear debris and inflammation at the site of an artificial joint in a patient. Treating osteolysis due to wear debris at a site of an artificial joint implant in a patient includes administering processed biological material at or proximate to the wear debris at the site of the artificial joint implant. In some embodiments, the processed biological material is injected into a tissue or combined with a graft material or implant.
In some embodiments, the biological material is harvested from a patient at a location different from where the processed biological material will be administered. For example, blood can be harvested from a patient's arm, processed in the device, and then administered at a site of inflammation near the patient's knee. In other embodiments, the biological material is harvested from a patient at a location that is the same as from where the processed biological material will be administered.
Embodiments of the present technology are further illustrated through the following non-limiting examples.
A device for processing a biological material, such as device 10 of
The needle 24 is inserted into an arm of a patient that has inflammation near a knee, the plunger 30 is drawn back, and blood is aspirated from the patient, through the filter 28, and into the syringe barrel 12. The blood is processed by inverting the device 10, and turning the plunger 30, which causes the paddle assembly 40 to turn and mix the polyacrylamide beads 26 with the blood. The polyacrylamide beads 26 activate components in the blood to generate anti-inflammatory cytokines. The processed blood is an autologous protein solution.
The needle 24 is inserted near the knee at the site of inflammation. Depressing the plunger 30 causes the autologous protein solution to flow out of the syringe barrel 12, through the filter 28, out the needle 24, and into the patient. The polyacrylamide beads 26 are excluded by the filter 28 from entering the patient. Pressing firmly on the plunger 30 causes the paddle assembly 40 to contact the filter 28 and collapse, which enables the plunger 30 to be further depressed to ensure all the autologous protein solution is delivered to the patient.
The device 10 described in Example 1 is selected. The needle 24 is inserted into an intramedullary area of a selected bone. The plunger 30 is drawn back and bone marrow is aspirated from the patient, through the filter 28, and into the syringe barrel 12. The bone marrow aspirate is processed by inverting the device 10, and turning the plunger 30, which causes the paddle assembly 40 to turn and mix the polyacrylamide beads 26 with the bone marrow aspirate. The polyacrylamide beads 26 absorb fluid from the bone marrow aspirate, which results in a processed composition comprising concentrated bone marrow aspirate. The needle 24 is then inserted back into the patient, and the plunger 30 is depressed to administer the concentrated bone marrow aspirate to the patient. The polyacrylamide beads 26 are excluded by the filter 28 from entering the patient. Pressing firmly on the plunger 30 causes the paddle assembly 40 to contact the filter 28 and collapse, which enables the plunger 30 to be further depressed to ensure all the autologous protein solution is delivered to the patient.
The device 10 described in Example 1 is selected. The needle 24 is inserted into an arm of a patient, the plunger 30 is drawn back, and blood is aspirated from the patient, through the filter 28, and into the syringe barrel 12. The needle 24 is removed from the outlet 22 and the outlet 22 is covered with a cap. The blood is processed by inverting the device 10, and turning the plunger 30, which causes the paddle assembly 40 to turn and mix the polyacrylamide beads 26 with the blood. The polyacrylamide beads 26 activate components in the blood to generate anti-inflammatory cytokines.
The cap is removed from the outlet 22, and a second filter, which has a pore size smaller than red blood cells, but larger than platelets, is coupled to the outlet. A new needle is coupled to the filter. The needle is inserted into the patient. Depressing the plunger 30 causes the processed blood to flow out the filter 28, through the second filter, through the needle, and into the patient. Because the second filter excludes red blood cells, platelet-rich plasma is administered to the patient. The polyacrylamide beads 26 are excluded by the filter 28 in the syringe barrel 12 from entering the patient. Pressing firmly on the plunger 30 causes the paddle assembly 40 to become compressed between the plunger 30 and the filter 28 and collapse, which enables the plunger 30 to be further depressed to ensure all the platelet-rich plasma is delivered to the patient.
The device 10 described in Example 1 is selected. The needle 24 is inserted into an arm of a patient, the plunger 30 is drawn back, and blood comprising macrophages is aspirated from the patient, through the filter 28, and into the syringe barrel 12. The blood comprising macrophages is processed by inverting the device 10, and turning the plunger 30, which causes the paddle assembly 40 to turn and mix the polyacrylamide beads 26 with the blood. Contact with the polyacrylamide beads 26 causes the macrophages to polarize into an anti-inflammatory M2 phenotype.
The needle 24 is inserted into a site of inflammation in the patient. Depressing the plunger 30 causes the M2 macrophages to flow out of the syringe barrel 12, through the filter 28, out the needle 24, and into the patient. The polyacrylamide beads 26 are excluded by the filter 28 from entering the patient. Pressing firmly on the plunger 30 causes the paddle assembly 40 to become compressed between the plunger 30 and the filter 28 and collapse, which enables the plunger 30 to be further depressed to ensure all the M2 macrophages are delivered to the patient.
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 disclosure. 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 disclosure, and all such modifications are intended to be included within the scope of the disclosure.
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