Patent Application
20210363478
This Patent Application claims priority from Italian Patent Application No. 102020000011926 filed on May 21, 2020, the entire disclosure of which is incorporated herein by reference.
The present invention relates to a device and to a method for the extraction of stem cells from adipose tissue.
As is known, stem cells are primitive, unspecialised cells, with the ability to transform into different types of cells in the body through a process called cell differentiation. They have been studied by researchers to treat certain diseases by exploiting their ductility.
Stem cells can be collected from different sources, such as the umbilical cord, amniotic sac, blood, bone marrow, placenta, and adipose tissues.
Among the various tissues listed above, adipose tissue is easily accessible and therefore forms the most convenient extraction region.
This tissue contains many types of cells, including connective cells, stroma and a small percentage (around 10%) of stem cells.
For this reason, it is necessary to extract a large amount of tissue (typically 6-10 grams) to be able to proceed with extraction of the stem cells. However, in some particularly thin subjects, it is difficult to obtain this amount of tissue.
The object of the present invention is to produce a device and a method for the extraction of stem cells from a limited amount of adipose tissue, in particular an amount of adipose tissue of around 1 gram. In particular, the object of the present invention is to produce a device that operates completely automatically.
Moreover, the object of the present invention is to produce a device and a method for the extraction of stem cells that makes it possible to control the experimental variables currently dependent on the single operator and capable of obtaining, with greater probability, homogeneous cells from a phenotypic, functional and genetic point of view.
The preceding object is achieved by the present invention, which relates to a device and to a method for the extraction of stem cells from adipose tissue as described in the appended claims.
The invention will now be illustrated with reference to the accompanying figures which represent a non-limiting embodiment thereof, wherein:
With reference to
The device 1 comprises the following units: a filtration system 6 (of a known type), a heat stirrer 11 (of a known type), a centrifugation system 7 (of a known type), a viewing system 8 (of a known type), and a plurality of containers 9 for the cell culture arranged on a supporting structure (rack) 10, a rack 12 for reagents 13, a buffer station 17 in which the container 4 can be temporarily arranged.
There is provided a loading station 18 in which a container 4 to be subjected to treatment is arranged.
There is provided a single container 23 (illustrated schematically) provided with a biological hood 24 and configured to contain the robotised handling system 2, the filtration system 6, the stirrer 11, the centrifugation system 7, the culture devices, the reagents rack 12, the viewing system 8 and the buffer station 17.
With reference to
The operations of the device 1 are performed according to what is illustrated below in
Advantageously, the adipose tissue collected from the patient is dissolved in an isotonic solution (input sample in
The container 4 is manually arranged on the loading station 18: subsequently, the electronic unit 20 automatically controls collection of the container 4 by means of the gripper 3 so that the container 4 is transferred to the filtration system 6, using 250 mcm nylon filters, where a first washing step with isotonic solutions is carried out by means of known techniques.
In this step, the lipoaspirate collected in the initial step is inserted (placed) on basket type nylon filters, in turn placed on Falcon tubes, and washed three times under gravity with isotonic solution.
Preferably, the washing liquid can be ejected with a high-pressure jet in order to facilitate removal of blood clots and tissue debris.
The lipoaspirate, purified of the blood clots and tissue debris, is transferred from the nylon filter support into a Falcon 4-a sterile container by means of the gripper 3 controlled by the control unit 20.
The electronic control unit 20 is subsequently designed to carry out a step in which an isotonic solution containing a predetermined amount of enzyme designed to start a cell disruption process is added to the lipoaspirate. This step is advantageously carried out by arranging the container 4 in the buffer station 17 and utilising the discharge suction system 5 carried by the gripper 3 and designed to collect the enzyme from the rack 12 of the reagents 13 and release the enzyme inside the container 4 (see
The electronic control unit 20 is designed to carry out a stirring and incubation step TA in which the solution of lipoaspirate and enzyme contained in the container 4 is pre-washed by the buffer station 17, supplied to the stirrer 11 where the solution of lipoaspirate and enzyme is stirred, thereby starting a chemical and mechanical breakdown process of the adipose tissue. The stirring operations take place, preferably but not exclusively, at 250 rpm and at a predetermined temperature of 37° C. corresponding to the temperature of the human body. This temperature is guaranteed by a thermoregulator (not illustrated).
The electronic unit 20 controls collection of the container 4-a from the stirrer 11 and re-transfers the container 4 to the filtration system 5 where a first filtering step is carried out, again by means of known techniques, such as using nylon filters.
A first microparticulate liquid phase containing the adipose stem cells is thus separated from a second semi-liquid phase of undigested adipose tissue.
The second semi-liquid phase of undigested adipose tissue is transferred by means of the gripper 3 into a first culture device C1 of a known type generally formed by a Petri plate or Petri capsule. This culture device C1 is arranged on the supporting rack 12 and is maintained in a controlled environment to obtain multiplication of the cells, thereby growing a first culture C1 of adipose stem cells.
The electronic unit 13 re-transfers the container 4-a to the centrifugation system 7 that receives the first microparticulate liquid phase and subjects it to a centrifugation operation CF producing a product that separates into three liquid phases and precisely:
The viewing system 8 detects an image of the three liquid phases arranged in the transparent container 4 and identifies on the image the separation zones Z1, Z2 between the first and second phases and the second and third phases, respectively. Knowing the separation zones Z1, Z2 allows the selective collection of the three phases, for example, by means of selective suction.
This suction is carried out using the suction and discharge system 5 carried by the gripper 3.
According to the present invention, the third liquid phase F3 (also called fat cake), after having been separated from the other phases, is transferred by means of the gripper 3 into a second culture device C2 of a known type generally formed by Petri plates or Petri capsules. This second culture device C2 is arranged on the supporting rack 12 and is maintained in a controlled environment to obtain multiplication of the stem cells thereby growing a second culture of adipose stem cells. Growth of the stem cells is controlled by means of observation, by the operator, with an optical microscope that is carried into position by the gripper 3. This microscope is associated with a viewing system for viewing images of the culture on the monitor.
After having eliminated the second liquid phase F2 with intermediate density (EX), a culture medium utilised for growth of the adipose stem cells is added to the first liquid phase F1 (pellet). The electronic unit 13 re-transfers the container containing the first liquid phase F1 (containing pellet+culture medium) to the centrifugation system 7 and subjects it to a centrifugation operation CF typically carried out at 1,2000 rpm for 5 minutes at room temperature producing a product that separates into two phases and precisely:
By means of selective suction the further second liquid phase F2-b is eliminated and culture medium is added to the further first liquid phase F1-b for resuspension of the pellet. The suspension containing the further first phase F1-b and the culture medium is transferred by the gripper 3 into a third culture device C3 of a known type, generally formed by a Petri plate or Petri capsule. This third culture device is arranged on the supporting rack 12 and is maintained in a controlled environment to obtain multiplication of the stem cells thereby growing a third culture of adipose stem cells. Also in this case, growth of the stem cells is controlled by means of observation, by the operator, with an optical microscope that is carried into position by the gripper 3.
The novelty of the present invention is represented by initiation of several cultures (three) of stem cells thereby maximising the yield of the sample collected.
In fact, the inventors of the present patent application have discovered that also the first phase, represented by undigested adipose tissue and which is normally eliminated, contains a sufficient number of stem cells to initiate a cell culture. The procedure carried out by the device illustrated above is completely automatic, as the operator requires only to arrange the sample in the loading position, after which all the operations for processing the sample are carried out by the device 1 without any human intervention. The operator only provides for collection of the culture devices.
| Number | Date | Country | Kind |
|---|---|---|---|
| 102020000011926 | May 2020 | IT | national |
