You’re using a public version of DrugPatentWatch with 5 free searches available | Register to unlock more free searches. CREATE FREE ACCOUNT

Last Updated: March 29, 2024

Claims for Patent: 10,472,599


✉ Email this page to a colleague

« Back to Dashboard


Summary for Patent: 10,472,599
Title:Microfluidic cell culture of patient-derived tumor cell spheroids
Abstract: Provided herein are methods for culturing patient-derived tumor cell spheroids in a three-dimensional microfluidic device. The method comprises mincing primary tumor sample in a medium supplemented with serum; treating the minced primary tumor sample with a composition comprising an enzyme; collecting tumor spheroids having a diameter of 10 .mu.m to 500 .mu.m from the enzyme treated sample; suspending the tumor spheroids in biocompatible gel; and culturing the tumor spheroids in a three dimensional microfluidic device. Methods for identifying an agent for treating cancer and microfluidic devices that allow for the simultaneous exposure of the cultured patient-derived primary tumor cell spheroids to a treatment of choice and to control treatment are also provided.
Inventor(s): Barbie; David (Andover, MA), Aref; Amir (Malden, MA), Barbie; Thanh (Andover, MA), Jenkins; Russell W. (Boston, MA), Wong; Kwok-kin (Arlington, MA)
Assignee: Dana-Farber Cancer Institute, Inc. (Boston, MA)
Application Number:15/540,346
Patent Claims:1. A method for culturing patient-derived tumor cell spheroids in a three-dimensional microfluidic device, the method comprising: mincing a primary tumor sample in a medium supplemented with serum; treating the minced primary tumor sample with a composition comprising an enzyme; collecting tumor spheroids having a diameter of 10 .mu.m to 500 .mu.m from the enzyme treated sample; suspending the tumor spheroids in biocompatible gel; and culturing the tumor spheroids in a three dimensional microfluidic device.

2. The method of claim 1, wherein the minced primary tumor sample is frozen in a medium supplemented with serum and thawed prior to treating with the composition comprising the enzyme.

3. The method of claim 1, wherein the collected tumor spheroids are frozen in a freezing medium and then thawed before suspending in the biocompatible gel.

4. The method of claim 1, wherein the minced primary tumor sample comprises tumor pieces in the size of about 1 mm.

5. The method of claim 1, wherein the tumor spheroids having a diameter of 10 .mu.m to 500 .mu.m are collected from the enzyme mix treated sample with the use of a sieve.

6. The method of claim 1, wherein the tumor spheroids having a diameter of 10 .mu.m to 500 .mu.m are collected by sieving the enzyme mix treated sample via 500 .mu.m and 10 .mu.m cell strainers to yield tumor spheroids having a diameter of 10 .mu.m to 500 .mu.m.

7. The method of claim 1, wherein the enzyme is collagenase.

8. The method of claim 1, wherein the composition comprising the enzyme comprises a serum-supplemented culture medium, insulin, a corticosteroid, an antibiotic, collagenase and optionally a growth factor.

9. The method of claim 1, wherein the minced primary tumor sample is treated with the composition comprising the enzyme in an amount or for a time sufficient yield a partial digestion of the minced primary tumor sample.

10. The method of claim 1, wherein the minced primary tumor sample is treated with the composition comprising the enzyme for 30 minutes to 15 hours at a temperature of 25.degree. C. to 39.degree. C.

11. The method of claim 1, wherein the three dimensional microfluidic device comprises: one or more fluid channels flanked by one or more gel cage regions, wherein the one or more gel cage regions comprises the biocompatible gel in which the tumor spheroids are embedded, and wherein the device recapitulates in vivo tumor microenvironment.

12. The method of claim 1, wherein the three dimensional microfluidic device comprises: a substrate comprised of an optically transparent material and further comprising i) one or more fluid channels; ii) one or more fluid channel inlets; iii) one or more fluid channel outlets; iv) one or more gel cage regions; and v) a plurality of posts; wherein all or a portion of each gel cage region is flanked by all or a portion of one or more fluid channels, thereby creating one or more gel cage region-fluid channel interface regions; each gel cage region comprises at least one row of posts which forms the gel cage region; and the one or more gel cage region has a height of at least 500 .mu.m.

13. The method of claim 12, wherein the one or more gel cage region has a height sufficient for at least 200-1000 .mu.m above the tumor cell spheroids.

14. The method of claim 12, wherein the gel cage region has a cuboidal shape.

15. The method of claim 1, wherein the tumor spheroids are cultured in the presence and absence of a test agent.

16. The method of claim 1, further comprising detecting a change in the tumor cell spheroid culture indicative of a condition that is likely to reduce proliferation and/or dispersion of the tumor cell spheroids in the presence of the first test agent as compared to the absence of the first test agent.

Make Better Decisions: Try a trial or see plans & pricing

Drugs may be covered by multiple patents or regulatory protections. All trademarks and applicant names are the property of their respective owners or licensors. Although great care is taken in the proper and correct provision of this service, thinkBiotech LLC does not accept any responsibility for possible consequences of errors or omissions in the provided data. The data presented herein is for information purposes only. There is no warranty that the data contained herein is error free. thinkBiotech performs no independent verification of facts as provided by public sources nor are attempts made to provide legal or investing advice. Any reliance on data provided herein is done solely at the discretion of the user. Users of this service are advised to seek professional advice and independent confirmation before considering acting on any of the provided information. thinkBiotech LLC reserves the right to amend, extend or withdraw any part or all of the offered service without notice.