Patent Publication Number: US-2021189312-A1

Title: Cell culture substrate and manufacturing method thereof

Description:
TECHNICAL FIELD 
     The present invention relates cell culture substrate and manufacturing method thereof. 
     BACKGROUND ART 
     Generally, in the field of drug development, a screening test is known in which a drug is administered to a cell mass (spheroid) cultured in a three-dimensional shape to measure its metabolic ability to the drug. In order to increase the efficiency of this metabolic test, in recent years it has been required to cultivate uniform spheroids with high viability using a culture container that can be conveniently prepared. As a container for spheroid culture, as disclosed in PTL 1, a substrate or the like having an adhesion region and an inhibition region for cells is used as a culture substrate. 
     CITATION LIST 
     Patent Literature 
     [PLT1] JP2007-269973A 
     SUMMARY OF INVENTION 
     Technical Problem 
     Resins being able to cultivate relatively uniform spheroids and having a property that can be used for an adhesive region or an inhibition region are special and limited (PLT1). It is difficult to synthesize such a special resin, and it takes a long time and high cost. 
     Several embodiments of the present invention have been made in view of such circumstances and provide a cell culture substrate which can be conveniently produced using readily available materials and can cultivate uniform spheroids with high viability. 
     Solution to Problem 
     According to some embodiments of the present invention, a cell culture substrate having an adhesive portion and a non-adhesive portion is provided, wherein the adhesive portion and the non-adhesive portion have a concave-convex shape, and the contact angle of pure water on the non-adhesive portion is larger than that of the adhesive portion. 
     The present inventors found out that it is possible to culture uniform spheroids with high viability by using a cell culture substrate comprising an adhesive portion having a concave-convex shape and highly hydrophobic non-adhesive portion having a concave-convex shape different from the adhesive portion even with readily available materials, and thus has come to complete the present invention. 
     Various embodiments of the present invention are exemplified below. Embodiments shown below may be combined with each other. 
     It is preferred that, pitch P 1  of the concave-convex shape of the adhesive portion is larger than pitch P 2  of the concave-convex shape of non-adhesive portion. 
     It is preferred that, the ratio P 1 /P 2  of the pitch P 1  and the pitch P 2  is 2 or more. 
     It is preferred that, at least a part of the adhesive portion is separated by a partition portion, and the non-adhesive portion is formed on the partition portion. 
     It is preferred that, the non-adhesive portion has a plurality of columnar convex portion, the pitch at which the columnar convex portion of the non-adhesive portion is formed is 50 to 2000 nm, the columnar convex portion of the non-adhesive portion has an upper surface area of 1600 nm 2  to 4 μm 2 , and the gap G 2  between two adjacent columnar convex portions is in the range of 10 to 1960 nm. 
     It is preferred that, the adhesive portion and the non-adhesive portion are made of a same material. 
     According to another embodiment of the present invention, a manufacturing method of the cell culture substrate is provided that includes a step of irradiating a photocurable resin composition coated on a substrate with an active energy ray to cure the resin composition to form concave-convex shapes of the adhesive portion and the non-adhesive portion. 
     It is preferred that, the concave-convex shapes of the adhesive portion and the non-adhesive portion are formed by a nanoimprint method using a mold. 
    
    
     
       BRIEF DESCRIPTION OF DRAWINGS 
         FIGS. 1A to 1C  show a cell culture substrate  1  according to one embodiment of the present invention, wherein  FIG. 1A  is a plan view,  FIG. 1B  is a cross-sectional view taken along the line A-A, and  FIG. 1C  is a cross-sectional view showing a pattern in which the concave-convex shape according to another embodiment is inverted from the case of  FIG. 1B . 
         FIGS. 2A to 2B  are enlarged views of a region X in  FIG. 1B  showing an adhesive portion  3  according to one embodiment of the present invention, wherein  FIG. 2A  is a plan view, and  FIG. 2B  is a cross-sectional view taken along the line B-B. 
         FIGS. 3A to 3B  are enlarged views of a region Y in  FIG. 1B  showing a non-adhesive portion  5  according to one embodiment of the present invention, wherein  FIG. 3A  is a plan view,  FIG. 3B  is a cross-sectional view taken along the line C-C. 
         FIGS. 4A to 4B  are cross-sectional views of the cell culture substrate  1  according to one embodiment of the present invention, wherein  FIG. 4A  shows an example having a partition portion  19 , and  FIG. 4B  shows an example without a partition portion. 
         FIGS. 5A to 5E  show a transparent base  23  provided with light shielding part  21 , wherein  FIG. 5A  is a plan view,  FIG. 5B  is a cross-sectional view taken along the line D-D, and  FIGS. 5C to 5E  show another example of the method of forming a light shielding pattern  3 . 
         FIGS. 6A to 6C  are cross-sectional views showing a first transferred resin layer forming step of the present invention. 
         FIGS. 7A to 7D  are cross-sectional views showing an adhesive portion resin layer forming step of the present invention. 
         FIGS. 8A to 8E  are cross-sectional views showing a composite resin layer forming step of the present invention. 
         FIG. 9  shows SEM images A to D of samples 1 to 4. 
     
    
    
     DESCRIPTION OF EMBODIMENTS 
     Preferred embodiments of the present invention are specifically described below with reference to  FIGS. 1 to 4 . 
     1. Cell Culture Substrate 
     As illustrated in  FIG. 1B , a cell culture substrate  1  according to one embodiment of the present invention comprises a base  7  and a resin layer  9  on at least one surface of the base  7 , and the resin layer  9  has an adhesive portion  3  and a non-adhesive portion  5 . The concave-convex shape of the adhesive portion  3  and the non-adhesive portion  5  shown in  FIG. 1B  may have a shape in which the concave and convex of only one of the adhesive portion  3  and non-adhesive portion  5  is reversed, or may have a shape as shown in  FIG. 1C  in which the concave and convex of both are reversed. 
     It is preferred that, the non-adhesive portion  5  is arranged in such a manner that it surrounds the adhesive portion  3 , and the resin layer  9  is divided into the region of adhesive portion  3  and the region of non-adhesive portion  5 . However, it is not necessarily surrounded without a break, and a part may be discontinued. 
     The shape of the region of the adhesive portion  3  is not particularly limited, and may be a circle, a polygon, etc. For example, an embodiment in which a square region as shown in  FIG. 1A  is formed is conceivable. 
     Further, as illustrated in  FIG. 4A , the cell culture substrate  1  may have a partition portion  19  that separates at least a part of the adhesive portion. Further, as illustrated in  4 B, the cell culture substrate  1  may not have the partition portion  19 . In order to prevent detachment of the cells from the base during replacement of the medium or the like, it is preferable to have the partition portion  19 . 
     &lt;Base  7 &gt; 
     The material of the base  7  is preferably, but not particularly limited to a transparent base such as a resin base and a quartz base. From the viewpoint of flexibility, a resin base is more preferable. A resin constituting the resin base is made of, for example, one selected from the group consisting of polyethylene terephthalate, polycarbonate, polyester, polyolefin, polyimide, polysulfone, polyether sulfone, cyclic polyolefin, and polyethylene naphthalate. Further, the base  7  is preferably in the form of a film having flexibility, and preferably has a thickness ranging from 25 to 500 μm. 
     &lt;Resin Layer  9 &gt; 
     A resin constituting the resin layer  9  is not particularly limited, but it is preferable that the resin layer  9  is made of an inexpensive resin that is relatively easy to obtain and synthesize, such as acrylic resin, methacrylic resin, styrene resin, olefin resin, polycarbonate resin, polyester resin, epoxy resin, and silicone resin. The types of the resin materials of the adhesive portion  3  and the non-adhesive portion  5  may be different, but from the viewpoint of easiness of manufacture and efficiency, it is preferable to be the same. 
     &lt;Adhesive Portion  3 &gt; 
     As illustrated in  FIG. 2 , adhesive portion  3  has a concave-convex shape formed by a plurality of adhesive convex portions  11  and adhesive concave portions  13 . The convex portion and the concave portion may be inverted shapes. 
     &lt;Adhesive Convex Portion  11  and Adhesive Concave Portion  13 &gt; 
     The shape of the adhesive convex portion  11  is not particularly limited, but examples thereof include a column shape (a circular column shape, a polygonal columnar shape, etc.), a truncated cone, a microlens, and the like. The shape of the adhesive concave portion  13  is also not particularly limited, but examples thereof include a hole hollowed out in a shape such as a column shape (a circular column shape, a polygonal columnar shape, etc.), a truncated cone, a microlens, and the like. 
     The pitch P 1  at which the adhesive convex portion  11  or the adhesive concave portion  13  is formed may be within a range having adhesiveness to a target cell, and is, for example, 2 to 50 μm, preferably 5 to 20 μm, and more preferably 7 to 15 μm. If the pitch P 1  is too small, cells are difficult to adhere. Also, if the pitch P 1  is too large, cells are difficult to form spheroids. Specifically, the pitch P 1  is, for example, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 25, 30, 35, 40, 45, 50 μm, and may be within the range between any two of the numerical values exemplified here. The concave-convex shape formed by the adhesive convex portion  11  and the adhesive concave portion  13  may be regular or irregular, but is preferably regular from the viewpoint of working efficiency. In the case where the concave-convex shape is formed regularly, the distance between the tips of many convex portions or concave portions constituting the concave-convex shape is defined as “pitch”. In the case where the concave-convex shape is formed irregularly, the average value of the distances between the tips of the many convex portions or concave portions constituting the concave-convex shape is defined as “pitch”. 
     The height H 1  of the adhesive convex portion  11  is not particularly limited, but is, for example, 1 to 20 μm, preferably 1 to 10 μm, more preferably 1 to 5 μm. If the height H 1  is too low, cells are less likely to form spheroids, and if it is too high, the adhesive convex portion  11  tends to collapse easily. 
     A typical example of the adhesive portion has a plurality of columnar convex portions. The area of the upper surface of the columnar convex portion of the adhesive portion may be within a range having adhesiveness to the target cell, and is, for example, 1 to 2400 μm 2 , preferably 16 to 360 μm 2 , more preferably 36 to 196 μm 2 . The gap G 1  between two adjacent columnar convex portions may be within a range having adhesiveness to a target cell, and is, for example, 1 to 49 μm, preferably 4 to 19 μm, more preferably 6 to 14 μm. 
     &lt;Non-Adhesive Portion  5 &gt; 
     As illustrated in  FIG. 3 , the adhesive portion  3  has a concave-convex shape formed by a plurality of non-adhesive convex portion  15  and non-adhesive concave portion  17 . The convex portion and the concave portion may be inverted. 
     Further, the contact angle of water on the non-adhesive portion  5  is not particularly limited but is larger than that of the adhesive portion  3 . If the contact angle is larger than that of the adhesive portion  3 , cells are difficult to adhere to the non-adhesive portion  5  and are easy to form spheroids. The contact angle of water on the non-adhesive portion  5  is, for example, 90 to 180°, preferably 105 to 180°, more preferably 110 to 180°, further preferably 115 to 180°. 
     &lt;Non-Adhesive Convex Portion  15  and Non-Adhesive Concave Portion  17 &gt; 
     The shape of the non-adhesive convex portion  15  is not particularly limited, but examples thereof include a column shape (a circular column shape, a polygonal columnar shape, etc.), a truncated cone, a microlens, and the like. The shape of the non-adhesive concave portion  17  is also not particularly limited, but examples thereof include a hole hollowed out in a shape such as a column shape (a circular column shape, a polygonal columnar shape, etc.), a truncated cone, a microlens, and the like. 
     The pitch P 2  at which the non-adhesive convex portion  15  or the non-adhesive concave portion  17  is formed is 50 to 2000 nm, preferably 100 to 1000 nm, more preferably 150 to 800 nm. If the pitch P 2  is too small, cells can not recognize the concave and convex, and there is no discrimination between adhesiveness and non-adhesiveness. If P 2  is too large, cells tend to adhere. Specifically, the pitch P 2  is, for example, 50, 60, 70, 80, 90, 100, 150, 200, 250, 300, 350, 400, 450, 500, 550, 600, 650, 700, 750, 800, 850, 900, 950, 1000, 1250, 1500, 1750, 2000 nm, and may be within the range between any two of the numerical values exemplified here. The concave-convex shape formed by the non-adhesive convex portion  15  and the non-adhesive concave portion  17  may be regular or irregular, but is preferably regular from the viewpoint of working efficiency. In the case where the concave-convex shape is formed regularly, the distance between the tips of many convex portions or concave portions constituting the concave-convex shape is defined as “pitch”. In the case where the concave-convex shape is formed irregularly, the average value of the distances between the tips of the many convex portions or concave portions constituting the concave-convex shape is defined as “pitch”. 
     The pitch P 1  of the concave-convex shape of the adhesive portion  3  is larger than the pitch P 2  of the concave-convex shape of the non-adhesive portion  5 . The larger the pitch, the smaller the contact angle of water and the higher the adhesiveness to cells tends to be. On the other hand, the smaller the pitch, the larger the contact angle of water and the lower the adhesiveness to cells tend to be. Therefore, by surrounding the region of the concave-convex shape with a large pitch by the region of the concave-convex shape with a small pitch, spheroid can be easily formed. Preferably, the ratio P 1 /P 2  of the pitch P 1  and the pitch P 2  is 2 or more, more preferably 5 or more, further preferably 10 or more. When P 1 /P 2  is large, there is a tendency that the difference in adhesiveness tends to be large, and it is possible to cultivate spheroids more efficiently because the cells are more likely to gather. The upper limit of P 1 /P 2  is not particularly specified, but is, for example, 200. 
     The height H 2  of the non-adhesive convex portion  15  is not particularly limited, but is, for example, 50 to 2000 nm. The height H 2  is preferably 100 to 1000 nm, and more preferably 150 to 800 nm. If the height H 2  is too low, cells tend to adhere, and if it is too high, the non-adhesive convex portion  15  tends to collapse easily. 
     A typical example of the the non-adhesive portion has a plurality of columnar convex portions, more specifically, a plurality of convex portions with circular column shape. The area of the upper surface of the columnar convex portion of the non-adhesive portion may be within a range in which the adhesion to the target cell is low, and is, for example, 1600 nm 2  to 4 μm 2 . This area is preferably 810 nm 2  to 1 μm 2 , more preferably 0.02 to 0.6 μm 2 . The gap G 2  between two adjacent columnar convex portions may be within a range in which the adhesion to the target cell is low, and is, for example, 10 to 1960 nm, preferably 60 to 960 nm, and more preferably 110 to 760 nm. 
     A fluorine atom-containing layer may be provided in such a manner that the fluorine atom-containing layer covers the non-adhesive convex portion  15  and non-adhesive concave portion  17 , fluorine atom-containing layer may contain a fluorine atom, and its thickness and composition are not limited. By providing the fluorine atom-containing layer it becomes difficult for the cells to adhere. The fluorine atom-containing layer preferably contains a fluorine-containing group. The fluorine-containing group is, in one example, a perfluoroalkyl group, more specifically a perfluoroalkylsilane group. The number of carbon atoms of the perfluoroalkyl group is, for example, 1 to 10, specifically 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, and it may be within the range between any two of the numerical values exemplified here, fluorine-containing group is preferably chemically bonded to the non-adhesive convex portion  15  and the non-adhesive concave portion  17 , or the inorganic film. In general, the inorganic film has high adhesiveness to the resin layer  9 , and the fluorine-containing group tends to form a strong chemical bond to the inorganic film. Therefore, by providing the inorganic film between the non-adhesive convex portion  15 , the non-adhesive concave portion  17  and the fluorine atom-containing layer, the fluorine atom-containing layer is firmly held on the non-adhesive convex portion  15  and the non-adhesive concave portion  17 . Examples of the inorganic film include an inorganic oxide film, an inorganic nitride film, an inorganic oxynitride film, and the like. Examples of the inorganic element constituting the inorganic film include silicon and aluminum. The inorganic film is, for example, a silicon dioxide film or an aluminum oxide film. The thickness of the inorganic film is not particularly limited but is, for example, 1 to 20 nm. 
     The fluorine atom-containing layer, in one example, can be formed by forming an inorganic film on the non-adhesive convex portion  15  and the non-adhesive concave portion  17 , and reacting the inorganic film with a fluorine-containing silane coupling agent. The fluorine-containing silane coupling agent is, for example, a perfluoroalkyltrialkoxy (methoxy, ethoxy, etc.) silane. Since even when a fluorine-containing silane coupling agent is allowed to act on the non-adhesive convex portion  15  and the non-adhesive concave portion  17  without forming an inorganic film, it is preferable to previously form the inorganic film on the non-adhesive convex portion  15  and the non-adhesive concave portion  17 . An example of the fluorine-containing silane coupling agent is OPTOOL DSX (manufactured by Daikin Industries, Ltd.). 
     &lt;Region of Adhesive Portion  3 &gt; 
     The area of the region of the adhesive portion  3  may be appropriately adjusted according to the type of cells to be cultured and the intended use of the spheroid, and the area is not particularly limited, but is, for example, 25 to 1000000 μm 2 , preferably 100 to 250000 μm 2 , more preferably 2500 to 40000 μm 2 . When the shape of the region of the adhesive portion  3  is a square, the length of one side is 5 to 1000 μm, preferably 10 to 500 μm, more preferably 50 to 200 μm. 
     &lt;Region of Non-Adhesive Portion  5 &gt; 
     If the region of the non-adhesive portion  5  is too large with respect to the region of the adhesive portion  3 , spheroids are difficult to form because the cells are difficult to move to the region of the adhesive portion  3 . Therefore, the ratio of the area of the region of the non-adhesive portion  5  to the total area of region of the adhesive portion  3  and the region of the non-adhesive portion  5  is preferably, for example, 80% or less, more preferably 50% or less, further preferably 25% or less. 
     &lt;Partition Portion  19 &gt; 
     As illustrated in  FIG. 4A , in the case of having the partition portion  19  that separates at least a part of the adhesive portion  3 , preferably, the partition portion  19  is arranged in such a manner that it surrounds the adhesive portion  3  to form a region of the adhesive portion  3 . However, it is not necessarily surrounded without a break, and a part may be discontinued. The shape of the region of the adhesive portion  3  is not particularly limited but may be a circle or a polygon such as a quadrangle. Preferably, the non-adhesive portion  5  is formed on the partition portion. The non-adhesive portion  5  may be formed on a part of the partition portion, and is preferably formed in such a manner that the non-adhesive portion  5  covers at least most of the upper surface of the partition portion  19 . The non-adhesive portion  5  may cover the entire surface of the partition portion  19 . 
     The height H 3  of the partition portion  19  is not particularly limited, but is, for example, 5 to 100 μm, preferably 10 to 50 μm, more preferably 15 to 25 μm. If the height H 3  is too low, the cells tend to be peeled off due to water flow or the like. If the height H 3  is too high, oxygen supply can not be sufficiently carried out and the cell viability is lowered. As illustrated in  FIG. 4A , the height H 3  is the height from the upper end of the adhesive convex portion  11  to the upper end of the partition portion including the non-adhesive portion. 
     2. Manufacturing Method of Cell Culture Substrate 
     Next, a manufacturing method of a cell culture substrate will be described with reference to  FIGS. 5 to 8 . 
     In one embodiment of the present invention, a manufacturing method of a cell culture substrate having a partition portion comprises: a non-adhesive portion transfer resin layer forming step, an adhesive portion resin layer forming step, and a composite resin layer forming step. 
     Each step will be described in more detail below. 
     (1) Non-Adhesive Portion Transfer Resin Layer Forming Step, 
     (1-1) First Transferred Resin Layer Forming Step 
     First, as illustrated in  FIG. 6A , a first photocurable resin composition is applied on a transparent base  23  having a light shielding part  21  as shown in  FIG. 5A  to form a first transferred resin layer  25 . 
     &lt;Transparent Base&gt; 
     The transparent base  23  is formed from a transparent material, such as a resin base, a quartz base, and a silicone base. The material is preferably, but not particularly limited to, a resin base. This is because use of a resin base enables a cell culture substrate obtained in a desired size (available in a large area) by the method of the present invention. A resin constituting the resin base is made of, for example, one selected from the group consisting of polyethylene terephthalate, polycarbonate, polyester, polyolefin, polyimide, polysulfone, polyether sulfone, cyclic polyolefin, and polyethylene naphthalate. The transparent base  23  preferably has flexibility, and when such a resin base is used, may be a laminate of same or different bases or a laminate of a resin composition in a film form on the resin base. The resin base preferably has a thickness ranging from 25 to 500 μm. 
     The light shielding part  21  provided in the transparent base  23  is a pattern utilized as a mask in the composite shape forming step. As illustrated in  FIGS. 8B to 8E , an adhesive portion  3  corresponding to the light shielding part  21 , a partition portion  19 , and a non-adhesive portion  5  on the partition portion are formed in a composite resin layer  45 . In an active energy ray irradiation step illustrated in  FIG. 8B , a region where active energy rays  29  is shielded by the light shielding part  21  becomes the adhesive portion  3 . The “active energy ray” is the generic name for energy lines capable of curing a photocurable resin composition, such as UV light, visible light, and electron beams. The shape of the light shielding part  21  is not particularly limited, but may be a square shape as illustrated in  FIG. 5A , a polygon such as a pentagon or a hexagon, a circle, or the like, and corresponds to the region of the adhesive portion  3 . 
     The light shielding part  21  may be formed by patterning after deposition of a light shielding material (for example, a metal material, such as Cr) on the transparent base  23  by sputtering or formed by printing a pattern of a light shielding material by a method, such as ink jet printing and screen printing. As illustrated in  FIGS. 5B to 5C , the light shielding part  21  may be formed on the side of a surface  23   a  of the transparent base  23  to apply the first photocurable resin composition, or as illustrated in  FIG. 5D , may be formed on a back side  23   b  of the transparent base  23 . The light shielding part  21 , as illustrated in  FIG. 5B , may be formed flush with the transparent base  23 , may be formed on a flat surface of the transparent base  23  as illustrated in  FIG. 5C , or may be mounted in the transparent base  23  as illustrated in  FIG. 5E . 
     &lt;First Photocurable Resin Composition&gt; 
     The first photocurable resin composition constituting the first transferred resin layer  25  contains a monomer and a photoinitiator and is cured by irradiation with an active energy ray. 
     Examples of the monomer include photopolymerizable monomers to form a acrylic resin, a methacrylic resin, a styrene resin, an olefin resin, a polycarbonate resin, a polyester resin, an epoxy resin, a silicone resin, and the like, and a photopolymerizable acrylic monomer and/or methacrylic monomer is preferred. 
     The photoinitiator is a component to be added to accelerate polymerization of a monomer and is preferably contained 0.1 parts by mass or more based on 100 parts by mass of the monomer. The upper limit of the photoinitiator content is not particularly defined but, for example, 20 parts by mass based on 100 parts by mass of the monomer. 
     The first photocurable resin composition of the present invention may contain components, such as a solvent, a polymerization inhibitor, a chain transfer agent, an antioxidant, a photosensitizer, a filler, and a leveling agent, without affecting the properties of the first photocurable resin composition. 
     The first photocurable resin composition may be manufactured by mixing the above components in a known method. The first photocurable resin composition may be applied on the transparent base  23  by a method, such as spin coating, spray coating, bar coating, dip coating, die coating, and slit coating, to form the first transferred resin layer  25 . 
     The first transferred resin layer  25  is generally a transparent resin layer and has a thickness from 100 nm to 1 mm and preferably from 5 to 500 μm. With such a thickness, it is easy to perform imprinting processing and it is possible to form a reverse pattern of a non-adhesive portion. 
     (1-2) Transfer and Curing Step 
     Then, as illustrated in  FIGS. 6A to 6C , with a first pattern  28  of a first mold  27  pressed against the first transferred resin layer  25 , the first transferred resin layer  25  is irradiated with the active energy ray  29  through the first mold  27 , and thereby the non-adhesive portion transfer resin layer  31  with the first pattern  28  transferred thereto is formed. 
     The first mold  27  has the first pattern  28 . In the present embodiment, the first pattern  28  is a desired pattern of a non-adhesive portion  5 . 
     The first mold  27  is made of a transparent material such as a resin base, a quartz base, and a silicone base, and can be formed of the same material as the transparent base  23 . 
     The first mold  27  may be pressed against the first transferred resin layer  25  at a pressure that allows transfer of the shape of the first pattern  28  to the first transferred resin layer  25 . 
     The first transferred resin layer  25  may be irradiated with the active energy ray  29  at an amount of the integral light to sufficiently cure the first transferred resin layer  25 . The amount of the integral light is, for example, 100 to 10000 mJ/cm 2 . By the irradiation with the active energy ray  29 , the first transferred resin layer  25  is cured to form, as illustrated in  FIG. 6C , the first reverse pattern  32  in which the first pattern  28  is inverted, that is, the non-adhesive portion transfer resin layer  31  on which the inverted pattern of the desired non-adhesive portion  5  is formed. 
     (2) Adhesive Portion Resin Layer Forming Step 
     (2-1) Second Transferred Resin Layer Forming Step 
     First, as illustrated in  FIG. 7A , a second photocurable resin composition is applied on the base  7  to form a second transferred resin layer  33 . 
     The above descriptions on the first photocurable resin composition apply to the second photocurable resin composition as long as not being inconsistent with the spirit. The type of the second photocurable resin composition may be same as or different from that of the first photocurable resin composition. The second transferred resin layer  33  obtained by applying the second photocurable resin composition is generally a transparent resin layer, and has a thickness of 1 μm to 1 mm, preferably 50 to 500 μm. With such a thickness, it is easy to perform imprinting processing and it is possible to form an adhesive portion. 
     (2-2) Transfer and Curing Step 
     Then, as illustrated in  FIGS. 7B to 7D , with a second pattern  36  of a second mold  35  pressed against the second transferred resin layer  33 , the second transferred resin layer  33  is irradiated with the active energy ray to cure the second transferred resin layer  33 , and thereby the adhesive portion resin layer  39  is formed. 
     The second mold  35  has the second pattern  36 . In the present embodiment, the second pattern  36  is a desired reverse pattern of an adhesive portion  3 . 
     When the base  7  is transparent, irradiation with the active energy ray  29  may be performed from the side of the base. The second mold  35  may be formed of a transparent material such as a resin base, a quartz base, a silicone base, or a metal material. 
     The second mold  35  may be pressed against the second transferred resin layer  33  at a pressure that allows transfer of the shape of the second pattern  36  to the second transferred resin layer  33 . 
     The second transferred resin layer  33  may be irradiated with the active energy ray  29  at an amount of the integral light to sufficiently cure the second transferred resin layer  33 . The amount of the integral light is, for example, 100 to 10000 mJ/cm 2 . By the irradiation with the active energy ray  29 , the second transferred resin layer  33  is cured to form, as illustrated in  FIG. 7D , the second reverse pattern  40  in which the second pattern  36  is inverted, that is, the adhesive portion resin layer  39  on which the desired non-adhesive portion  5  is formed. 
     (3) Composite Resin Layer Forming Step 
     (3-1) Third Transferred Resin Layer Forming Step 
     First, as illustrated in  FIG. 8A , a third photocurable resin composition is applied on the adhesive portion resin layer  39  to form a third transferred resin layer  41 . 
     The above descriptions on the first photocurable resin composition apply to the second photocurable resin composition as long as not being inconsistent with the spirit. The type of the third photocurable resin composition may be same as or different from that of the first photocurable resin composition, and may be same as or different from that of the second photocurable resin composition, the third transferred resin layer  41  obtained by applying the third photocurable resin composition is generally a transparent resin layer, and has a thickness of 10 μm to 1 mm, preferably 50 to 500 μm. With such a thickness, it is easy to perform imprinting processing and it is possible to form a partition portion and a non-adhesive portion. 
     (3-2) Transfer and Curing Step 
     Then, as illustrated in  FIGS. 8B to 8E , with a non-adhesive portion transfer resin layer  31  as a mold pressed against the third transferred resin layer  41 , the third transferred resin layer  41  is irradiated with the active energy ray to cure the third transferred resin layer  41 , and thereby the composite resin layer  45  is formed. 
     The non-adhesive portion transfer resin layer  31  may be pressed against the third transferred resin layer  41  at a pressure that allows transfer of the shape of the non-adhesive portion transfer resin layer  31  to the third transferred resin layer  41 . 
     The third transferred resin layer  41  is irradiated with the active energy ray  29  the from the non-adhesive portion transfer resin layer  31 . 
     The third transferred resin layer  41  may be irradiated with the active energy ray  29  at an amount of the integral light to sufficiently cure the third transferred resin layer  41 . The amount of the integral light is, for example, 100 to 10000 mJ/cm 2 . By the irradiation with the active energy ray  29 , in the region not shielded by the light shielding part  21 , the third photocurable resin composition filled in the gap of the adhesive portion resin layer  39  is cured and the third transferred resin layer  41  to which the reverse pattern of the non-adhesive portion transfer resin layer  31  was transferred is cured, and thereby the composite resin layer  45  is formed. In this step, the partition portion  19  shown in  FIG. 8E  and the non-adhesive portion  5  on the partition portion  19  are formed in the region where the third photocurable resin composition was cured. On the other hand, the adhesive portion  3  remains intact in the region where the active energy ray  29  was shielded by the light shielding part  21  and the third photocurable resin composition was not cured. 
     Then, as illustrated in  FIGS. 8D to 8E , the non-adhesive portion transfer resin layer  31  is removed and third photocurable resin composition  42  remaining on the adhesive portion  3  is removed with solvent to obtain the structure shown in  FIG. 8E , and the production of the cell culture substrate is completed. 
     By using the composite resin layer  45  formed above, it is possible to prepare a mold having the reverse pattern of the composite resin layer  45 , and by using this mold, a cell culture substrate having the same pattern as that of the composite resin layer  45  can be prepared at once. 
     In the case of not having the partition portion portion, it is possible to manufacture the cell culture substrate as shown in  FIG. 4B  by using a mold having the adhesive portion  3  and the reverse pattern of the non-adhesive portion  5 . 
     EXAMPLES 
     1. Preparation of Cell Culture Substrate Sample 
     Hereinafter, the preparation of the cell culture substrate sample used for cell culture and the evaluation of drug metabolism will be described. 
     &lt;Preparation of Photocurable Resin Composition&gt; 
     First, a photocurable resin composition was prepared by blending a photopolymerizable monomer and a photoinitiator in the proportions shown below. 
     Photopolymerizable Monomer: 
     Ethylene oxide modified trimethylolpropane triacrylate (Manufactured by Osaka Organic Chemical Industry Ltd.; Name of product: Viscoat #360): 50 parts by mass 
     Ethylene oxide modified bisphenol A diacrylate (Manufactured by Osaka Organic Chemical Industry Ltd.; Name of product: Viscoat #700HV): 20 parts by mass 
     Tripropylene glycol diacrylate (Manufactured by Osaka Organic Chemical Industry Ltd.; Name of product: Viscoat #310HP): 30 parts by mass 
     Photoinitiator: 
     1-hydroxycyclohexyl phenyl ketone (Manufactured by BASF Japan; product name: Irgacure 184): 5 parts by mass 
     &lt;Preparation of Sample&gt; 
     [Sample 1] (Example 1) 
     (Formation of Non-Adhesive Portion Transfer Resin Layer) 
     As illustrated in  FIG. 5 , the photocurable resin composition prepared above was applied to the PET base  47  provided with the light shielding part  21  as a plurality of squares at a thickness of 10 μm with a bar coater, and a lamination was carried out on a mold of nanopillar having a circular column shape (pitch: 150 nm, height: 250 nm, diameter: 100 nm) with a roller from above in such a manner that the coated resin surface is pressed against the mold. Thereafter UV irradiation was performed from the mold side at an amount of the integral light of 500 mJ/cm 2  to cure the photocurable resin composition. The mold and the resin-cured PET base were peeled off to prepare a nanohole transfer resin layer having the reverse shape of the mold. 
     (Formation of Adhesive Portion Resin Layer) 
     The photocurable resin composition prepared above was applied to the PET base at a thickness of 10 μm with a bar coater, and a lamination was carried out on a mold of nanohole having a hexagonal columnar shape (honeycomb) (pitch:12 μm, depth: 5 μm, parallel two side width: 17 μm) with a roller from above in such a manner that the coated resin surface is pressed against the mold. Thereafter, UV irradiation was performed from the PET base side at an amount of the integral light of 500 mJ/cm 2  to cure the photocurable resin composition. The mold and the resin-cured PET base were peeled off to prepare a nanopillar transfer resin layer having the reverse shape of the mold. 
     (Formation of Composite Resin Layer) 
     The photocurable resin composition prepared above was applied to the nanopillar transfer resin layer at a thickness of 10 μm with a bar coater, and a lamination was carried out on the nanohole transfer resin layer from above using the nanohole transfer resin layer as a mold in such a manner that the coated resin surface is pressed against the nanohole transfer resin layer. Thereafter. UV irradiation was performed from the nanohole transfer resin layer at an amount of the integral light of 500 mJ/cm 2  to cure the photocurable resin composition. The nanohole transfer resin layer and the nanopillar transfer resin layer were peeled off, and the uncured photocurable resin composition remaining on the nanopillar transfer resin layer was removed with isopropyl alcohol to prepare a cell culture substrate. 
     [Sample 2] (Comparative Example 1) 
     A cell culture substrate was prepared in the same manner as in the composite resin layer forming step of Sample 1, except that instead of using the nanohole transfer resin layer as the mold, a flat one having the same light shielding part  21  in lattice shape and not having the concave-convex shape was used. 
     [Sample 3] (Comparative Example 2) 
     A cell culture substrate was prepared only by the adhesive portion resin layer forming step of Sample 1. 
     [Sample 4] (Comparative Example 3) 
     The photocurable resin composition prepared above was applied to the PET base at a thickness of 10 μm with a bar coater, and UV irradiation was performed from the PET base side at an amount of the integral light of 500 mJ/cm 2  to cure the photocurable resin composition. 
     &lt;Measurement of Each Part of Sample 1&gt; 
     A part of Sample 1 was excised, the shape was observed using a scanning electron microscope (model: JSM-7800F, manufactured by JEOL Ltd.), and each part was measured using software (PC-SUM) attached to the same microscope. The results for the adhesive portion and the non-adhesive portion are shown in Table 1, and the results for the partition portion are shown in Table 2. In the sample 1, the upper surface area of the partition portion is substantially equal to the area of the region of the non-adhesive portion. 
     
       
         
           
               
               
               
             
               
                   
                 TABLE 1 
               
               
                   
                   
               
               
                   
                 Adhesive Portion 
                 Non-adhesive Portion 
               
               
                   
                   
               
             
            
               
                   
               
            
           
           
               
               
               
            
               
                 Shape 
                 Hexagonal Column 
                 Circular Column 
               
            
           
           
               
               
               
               
               
            
               
                 Pitch 
                 12 
                 μm 
                 150 
                 nm 
               
               
                 Height 
                 5 
                 μm 
                 250 
                 nm 
               
               
                 Width/Diameter 
                 10 
                 μm 
                 100 
                 nm 
               
               
                 Upper Surface Area 
                 195 
                 μm 2   
                 10000 
                 πnm 2   
               
               
                   
               
            
           
         
       
     
     
       
         
           
               
               
             
               
                   
                 TABLE 2 
               
               
                   
                   
               
               
                   
                 Partition Portion 
               
               
                   
                   
               
             
            
               
                   
               
            
           
           
               
               
               
               
            
               
                   
                 Width 
                 3 
                 μm 
               
               
                   
                 Height 
                 12 
                 μm 
               
               
                   
                 Per Unit Area of Separated 
                 95 × 95 
                 μm 2   
               
               
                   
                 Adhesion Portion 
               
               
                   
                 Per Unit Area of Upper Surface 
                 2000 
                 μm 2   
               
               
                   
                 of Partition Portion 
               
               
                   
                   
               
            
           
         
       
     
     &lt;Measurement of Contact Angle of Water&gt; 
     With respect to the obtained Sample 1, 0.5 μl of ion-exchanged water was dropped on the surface of the adhesive portion and the non-adhesive portion of Sample 1, and the contact angle of water (water contact angle) was measured at 25° C. using a contact angle measuring device (manufactured by dataphysics) and found to be 100° and 115° respectively. 
     2. Cell Culture and Drug Metabolism 
     The results of the cell culture and drug metabolism using the cell culture substrate of the present invention will be described below. 
     &lt;Cell Culture Method&gt; 
     The cell culture substrate was placed on the bottom of a 6 -well plate (manufactured by Thermo Fisher Scientific) and immersed in 70% ethanol for 1 hour. Then, it was washed three times with PBS having a pH of 7.4 (hereinafter the same) and dried. 
     Next, rat hepatocytes were suspended in DMEM medium (manufactured by Thermo Fisher Scientific), seeded in a well plate at 1×10 5  cells/well and cultured at 37° C. under 5% CO 2  for 14 days. The medium was exchanged the next day of culture, and thereafter it was exchanged every other day. 
     &lt;Aggregated Shape&gt; 
     In order to investigate the formation of spheroids, the aggregated shape after 14 days after seeding was observed using SEM. SEM images in the case of using Samples 1 to 4 are shown in  FIGS. 9A to 9D . 
     In Sample 1, the cells aggregated in a spherical shape in the lattice, the size of each aggregate was close, and uniform spheroids were formed. In Sample 2, the cells aggregated to some extent but not in a spherical shape as they were crossing the lattice, and it can not be said that their sizes were uniform. Unlike Sample 1, it is presumed that it may be caused by not having a non-adhesive portion on the lattice. In Sample 3, although the cells aggregated, they were only somewhat rounded and their sizes were largely different from each other. It is presumed that this is because the adhesive portion was not surrounded by a non-adhesive portion and there was no partition portion. In sample 4, the cells only spread thinly. 
     &lt;Evaluation of Drug Metabolism&gt; 
     The evaluation of drug metabolism was performed 1, 7 and 14 days after seeding. After 1, 7 and 14 days, replace medium with induction medium (3-MC 0.333 mM) and incubate for 24 hours. Subsequently, the medium was replaced with a reaction medium (PBS 50 ml, Dicumarol 25 μM, Probenecid 2 mM, ethoxyresorufin 20 μM) heated to 37° C. after 60 minutes of incubation, the pH was adjusted to 7.4 with HCl. 200 μl of supernatant and 200 μl of blank (unreacted reaction medium) were placed in a 96-well plate, and the amount of fluorescence [530/590] was measured with a fluorescence plate reader. 
     The evaluation of drug metabolism of Samples 1 to 4 is shown in Table 3. 
     
       
         
           
               
               
             
               
                   
                 TABLE 3 
               
             
            
               
                   
                   
               
               
                   
                 Amount of Drug Metabolism (μM/1 × 10 5  cells) 
               
            
           
           
               
               
               
               
               
            
               
                   
                 Samples 
                 1 day later 
                 7 days later 
                 14 days later 
               
               
                   
                   
               
            
           
           
               
               
               
               
               
            
               
                 Example 1 
                 1 
                 4.8 
                 6.4 
                 7.8 
               
               
                 Comparative 
                 2 
                 2.5 
                 3.2 
                 6.6 
               
               
                 Example 1 
               
               
                 Comparative 
                 3 
                 3.7 
                 4.0 
                 5.2 
               
               
                 Example 2 
               
               
                 Comparative 
                 4 
                 2.7 
                 2.5 
                 2.6 
               
               
                 Example 3 
               
               
                   
               
            
           
         
       
     
     In sample 1, it is estimated that the amount of drug metabolism is large, and the oxygen supply is sufficiently carried out on the spheroid being formed. In Sample 2, although the amount of drug metabolism was relatively large, it was inferior to Sample 1. In Sample 3, the amount of drug metabolism was as little as 30 to 40% of Sample 1. In Sample 4, the amount of drug metabolism was greatly reduced. 
     REFERENCE SIGNS LIST 
       1 : Cell Culture Substrate,  3 : Adhesive Portion,  5 : Non-Adhesive Portion,  19 : Partition portion.  29 : Active Energy Ray, P 1 : Pitch of Concave-Convex Shape of Adhesive Portion, P 2 : Pitch of Concave-Convex Shape of Non-Adhesive Portion. G 2 : Gap Between Two Adjacent Columnar Convex Portions