Cell and tissue culture device with controlled culture fluid...

Chemistry: molecular biology and microbiology – Apparatus – Including condition or time responsive control means

Reexamination Certificate

Rate now

  [ 0.00 ] – not rated yet Voters 0   Comments 0

Details

C435S286600, C435S297100, C435S297500

Reexamination Certificate

active

06576458

ABSTRACT:

The invention relates to the field of cell and tissue culture with the help of a culture fluid or nutrient medium.
This invention more particularly relates to devices and methods for cell and tissue culture in which the culture fluid (or nutrient) is set into motion so as to achieve a dynamic culture. Such devices usually apply either a technique for directly stirring the culture fluid in the culture volume or a technique providing permanent flow of the fluid through a specific circuit.
These techniques for fluid flow are difficult to control because culture conditions change over time. Actually, the low cell concentration which exists at the beginning of the culture process, requires a quasi-static environment, and therefore a very low culture fluid flow rate, whereas cell multiplication or tissue growth needs a rapidly increasing flow rate.
Maintaining adequate conditions during the whole culture process requires either the use of several suitable devices, at different stages of the culture's growth, respectively, and this involves many handling operations, or complex and often cumbersome means, which limit, even precludes observation of the culture's development with a microscope. These handling operations and means are all the more complex as the culture process should be carried out in a sterile environment which requires highly qualified personnel, and this therefore increases the cost for each culture. Furthermore, because of their price, these devices should be reusable, which imposes complete sterilization before each new culture, and maintenance operations.
The object of the invention is therefore to overcome all or part of the aforementioned drawbacks.
For this purpose, it provides a cell and tissue culture device which initially comprises a pressurization circuit capable of delivering at least a selected gas under a selected pressure, at least a culture chamber accommodating supporting means for at least a deformable membrane forming inside the chamber an interface between first and second portions with variable complementary volumes and supplied with culture fluid by a first tank and with selected gas by the pressurization circuit, respectively; the first portion further receiving the cells or tissues to be grown. The device further comprises control means capable of determining, according to selected criteria relating to the type of culture to be achieved, the gas to be fed into the second portion, its pressure and the time for feeding it in, and of controlling access to the first and second portions of the chamber so as to control together the shape of the membrane, culture fluid supply and flow of this fluid in the first portion.
By varying the pressure of the gas in the second portion, the shape of the membrane(s) may be changed, and the culture fluid may be forced to flow in the first portion of the chamber. For example, overpressurization phases may be alternated with depressurization phases in the second portion of the chamber in order to cause oscillation of the membrane(s).
Thus, for example, defining for each type of culture, a series of parameter n-tuples each including at least a selected gas, a pressure for this gas, a time for feeding in this gas, a culture fluid flow rate and a time for feeding in this fluid, is sufficient for controlling the growth of this culture. However, more complex modes may be considered which are based on adapting the multiple parameters from physical measurements, such as temperature measurements, or measurements of the proportion of molecular species or even pH measurements, carried out in the chamber and/or in the pressurization circuit.
All these parameters may be stored and/or calculated in the control means. They may be also changed through reprogramming.
Conducting pressure measurements in the culture chamber, or measurements of culture fluid level in the culture chamber or even calorimetric measurements for quantifying growth of certain cultures, or even redox potential measurements may also be considered.
In the case of a single membrane device, providing a supramembrane above the latter may be advantageous, in order to delimit between them at least an intermediate area supplied with gas by the pressurization circuit and able to discharge at least a portion of this gas, wherein the control means are configured so as to determine, according to selected criteria, the gas to be fed into the intermediate area, its pressure and time for feeding it in, and for controlling access to the inlet and outlet of the intermediate area so as to control together the shapes of the membrane and supramembrane and culture fluid flow in the first portion. This supramembrane may be firmly secured to the membrane at a multiplicity of selected locations, so as to subdivide the intermediate area into a plurality of communicating cellular cavities of variable volumes.
The intermediate area may optionally be fed with a gas other than the one fed into the second portion.
In a preferred embodiment of the device according to the invention, supporting means are configured so as to support a multiplicity of independent membranes, which may be gathered together in two, three, four or even more independent groups. Thus, according to the type of programming for the control means and according to the number of membrane groups, it is possible to generate a large number of fluid flow modes in the first portion, for example, an essentially “horizontal” flow, an essen-tially “vertical” flow, a combination of vertical and horizontal flows, or even a “zig-zag” flow.
The number of flow modes may further be increased by providing the first portion of the culture chamber on the opposite side of the second portion, with a deformable pocket or one or more auxiliary deformable membranes supplied with gas, preferably with the selected gas by the pressurization circuit. However, it may be a different complementary gas, (in this case, it is clear that the pressurization circuit should include two parallel branches supplied with two different gases).
If several auxiliary membranes are used, they may be subdivided into independent groups (two, three, four or more), as previously explained for the other membranes. Each group may also be subdivided into independent subgroups, subject to adaptation of the gas supply mode for the groups (addition of supply ducts and valves).
Moreover, and always in this case, partitioning means may be provided in the central part of the first portion, defining within the latter, culture cavities each extending from a group of membranes to a group of auxiliary membranes, wherein each cavity is supplied with culture fluid. These partitioning means may include for example partitions made of a porous material to the culture fluid, but impervious to cells and tissues, so that only the culture fluid flows from one cavity to another.
On the other hand, the first portion may accommodate at least a deformable side membrane forming an interface between a side portion and the portion containing the cells or tissues, wherein the side portion is supplied with gas by the pressurization circuit and may discharge at least a portion of this gas. Of course, in this case, the control means are configured so as to determine, according to selected criteria, the pressure and the time for feeding in the gas, and for controlling access to the inlet and outlet of the side portion in order to control the shape of the side membrane(s). The gas introduced into this side portion may either be the gas selected for feeding the second portion, or another selected gas (with an additional branch in the pressurization circuit).
Preferably, each membrane, side membrane, auxiliary membrane and pocket is made of a porous material, at least in the direction pointing to the first portion which contains the cells or tissues to be grown, so that the selected gas may at least partially penetrate the first portion.
The device may comprise several culture chambers, for instance two or three, or even more. These chambers may be accommodated in a compartment and/or be exter

LandOfFree

Say what you really think

Search LandOfFree.com for the USA inventors and patents. Rate them and share your experience with other people.

Rating

Cell and tissue culture device with controlled culture fluid... does not yet have a rating. At this time, there are no reviews or comments for this patent.

If you have personal experience with Cell and tissue culture device with controlled culture fluid..., we encourage you to share that experience with our LandOfFree.com community. Your opinion is very important and Cell and tissue culture device with controlled culture fluid... will most certainly appreciate the feedback.

Rate now

     

Profile ID: LFUS-PAI-O-3140897

  Search
All data on this website is collected from public sources. Our data reflects the most accurate information available at the time of publication.