Tracking Bispecific Antibody-Induced T Cell Trafficking Using Luciferase-Transduced Human T Cells

Madelyn Espinosa-Cotton; Hong-Fen Guo; Nai-Kong V. Cheung

doi:10.3791/64390

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Podsumowanie
Streszczenie
Wprowadzenie
Protokół
Wyniki
Dyskusje
Ujawnienia
Podziękowania
Materiały
Odniesienia
Przedruki i uprawnienia

Podsumowanie

Here, we describe a method for transducing human T cells with luciferase to facilitate in vivo tracking of bispecific antibody-induced T cell trafficking to tumors in studies to evaluate the anti-tumor efficacy and mechanism of T cell-engaging bispecific antibodies.

Streszczenie

T cell-engaging bispecific antibodies (T-BsAbs) are in various stages of preclinical development and clinical testing for solid tumors. Factors such as valency, spatial arrangement, interdomain distance, and Fc mutations affect the anti-tumor efficacy of these therapies, commonly by influencing the homing of T cells to tumors, which remains a major challenge. Here, we describe a method to transduce activated human T cells with luciferase, allowing in vivo tracking of T cells during T-BsAb therapy studies. The ability of T-BsAbs to redirect T cells to tumors can be quantitatively evaluated at multiple time points during treatment, allowing researchers to correlate the anti-tumor efficacy of T-BsAbs and other interventions with the persistence of T cells in tumors. This method alleviates the need to sacrifice animals during treatment to histologically assess T cell infiltration and can be repeated at multiple time points to determine the kinetics of T cell trafficking during and after treatment.

Wprowadzenie

T cell-engaging bispecific antibodies (T-BsAbs) are engineered antibodies used to provide artificial specificity to polyclonal T cells by engaging T cells through one binding arm and a tumor antigen through another binding arm. This technology has been successfully applied to hematological cancers (CD19-targeting blinatumomab¹), and numerous T-BsAbs are in preclinical and clinical development for a variety of solid tumors as well². T-BsAbs engage polyclonal T cells in a major histocompatibility complex (MHC)-independent manner, and therefore even tumors that downregulate human leukocyte antigens (HLAs) are susceptible to this type of therapy³^,⁴. T-BsAbs have been developed in dozens of different formats, with differences in the valency and spatial arrangement of the T cell and tumor binding arms, interdomain distances, and the inclusion of an Fc domain, which affects the half-life and can induce effector functions if present⁵. Previous work in our lab has shown that these factors significantly affect the anti-tumor efficacy of T-BsAbs, with up to 1,000-fold differences in potency⁶. Through this work, we identified the IgG-[L]-scFv format as the ideal platform for T-BsAbs (see Representative Results section for more detail regarding T-BsAb formats), and have applied this platform to targets including GD2 (neuroblastoma), HER2 (breast cancer and osteosarcoma), GPA33 (colorectal cancer), STEAP1 (Ewing Sarcoma), CD19 (B cell malignancies), and CD33 (B cell malignancies)⁷^,⁸^,⁹^,¹⁰^,¹¹^,¹²^,¹³.

One of the major challenges to successfully implementing T-BsAb therapy in solid tumors is overcoming an immunosuppressive tumor microenvironment (TME) to drive T cell trafficking to tumors¹⁴. The factors affecting T-BsAb efficacy described above have a significant impact on the ability of T-BsAbs to effectively induce T cell homing to tumors, but this effect is difficult to evaluate in an in vivo system in real time. This manuscript provides a detailed description of the use of luciferase-transduced T cells in preclinical studies of T-BsAbs to evaluate T cell trafficking to various tissues in experimental immunocompromised mouse models during treatment. The overall goal of this method is to provide a means to evaluate T cell infiltration in tumors and other tissues, as well as real-time insight into T cell homing kinetics and persistence, without the need to sacrifice animals during treatment. For the increasing number of researchers focusing on cellular immunotherapies, the ability to track T cells in vivo in preclinical animal models is crucial. We aim to provide a thorough, detailed description of the method we have employed for tracking luciferase-transduced T cells to enable other researchers to easily replicate this technique.

Protokół

The following procedures have been evaluated and approved by Memorial Sloan Kettering's Institutional Animal Care and Use Committee.

1. Transfection of 293T cells with luciferase and harvest of viral supernatant

Culture of 293T cells
1. Prepare media by adding the following to a liter of DMEM each: 110 mL of heat-inactivated fetal bovine serum (FBS), 11 mL of penicillin-streptomycin.
2. Thaw 5 x 10⁶ 293T cells and transfer them into a T175 flask with the media prepared as described above.
3. Split the 293T cells 1:10 every 3 days for 6 days. Do not allow the cells to become more than 90% confluent.
Transfection of 293T cells
NOTE: The following quantities of reagents are calculated for transfecting one T175 flask of 293T cells. Adjust accordingly if more flasks are to be transduced.
1. Transfer 1.5 mL of media to each of the two 50 mL tubes using a pipette. To one tube, add 10 µg of VSV-G plasmid, 20 µg of Gag/pol, and 20 µg of click beetle red TD tomato (CBR-TDR) luciferase plasmid and mix. To the other tube, add 100 µL of DNA in vitro transfection reagent and mix. Incubate both tubes at room temperature (RT) for 5 min.
  NOTE: All plasmids described in this manuscript were provided by Dr. Vladimir Ponomarev.
2. Transfer the media containing the DNA in vitro transfection reagent dropwise to the tube containing the DNA plasmids (over approximately 30 s) and mix gently with a pipette. Incubate at RT for 20 min.
3. During this 20 min incubation, detach the 293T cells by adding 5-10 mL of 0.05% trypsin. Once the cells have detached, add 10 mL of media and centrifuge at 800 x g for 5 min. Resuspend the cells in 1.5 mL of media.
4. Add the media containing the DNA in vitro transfection reagent and the DNA plasmids to the 293T cells and incubate at 37 °C for 30 min.
5. Transfer to a T175 flask and add 18 mL of media. Incubate at 37 °C overnight.
6. The next day, carefully aspirate the media with a glass pipette without detaching the cells. Replace with 18 mL of fresh media. Incubate at 37 °C overnight in an incubator.
Harvesting viral supernatant
1. Remove the viral supernatant using a pipette put on ice. Centrifuge at 800 x g for 5 min to pellet the cells and debris.
  NOTE: If the cell pellet is large, the cells were likely disrupted from the flask when the supernatant was removed. These cells can be plated again in a new flask with fresh media.
2. Filter the viral supernatant using a 0.22 µm filter.
3. Use the viral supernatant immediately. Keep it on ice or at 4 °C for up to 24 h, or freeze it at -80° C for long-term storage.

2. Expansion and transduction of activated human T cells with luciferase

Activation of human T cells in vitro
1. Wash the beads by adding 10 mL of phosphate buffered saline (PBS) containing 0.1% bovine serum albumin (BSA) and 2 mM ethylenediaminetetraacetic acid (EDTA) to a sterile 15 mL tube, adding beads (one bead per two T cells), placing in a magnet rack for 2 min, and suctioning out the PBS.
2. Prepare media as described in step 1.1.1, then add IL-2 to a final concentration of 30 IU/mL and add the washed beads. Make 2.5 mL of media for every two million T cells to be activated.
3. Count the T cells (freshly purified or previously purified, frozen, thawed, and washed) using a hemocytometer and trypan blue stain. Add T cells to the media prepared in step 2.1.2 and gently invert the tube to mix. The T cells will expand at least 20x depending on the source and general health of the cells. Determine the number of T cells to activate by calculating the number needed to treat the mice and dividing by 20. Here, 20 x 106 T cells per mouse were used based on preliminary experiments.
4. Plate 2.5 mL of media containing two million T cells, beads, and IL-2 in each well of a 24-well tissue culture plate. Culture at 37 °C in a humidified 5% CO₂ incubator.
5. Examine the T cells under a 20x microscope every day for the next 3 days to determine when to transduce with luciferase. The cells are ready when they clump together and deplete the media, turning it from red/pink to light orange.
Preparation of retronectin plates
NOTE: Retronectin is used to coat the plates used in the transduction as it enhances gene transduction¹⁵.
1. Add 2 mL of 20 µg/mL retronectin in PBS to a well of an untreated 6-well plate. Incubate for 2 h at RT or 1 h at 37 °C. One retronectin-coated well is required for every two million T cells to be transduced.
2. Aspirate the retronectin without scratching the bottom of the plate.
3. Add 3 mL of 2% BSA in PBS (sterile filtered) per well in the 6-well plate. Incubate for 30 min at RT.
Spinoculation
1. Aspirate the BSA without scratching the bottom of the plate.
2. Wash the wells once with 3 mL of PBS per well. Continue or replace with fresh PBS and leave the plate covered at 4 °C overnight.
3. Add 2 mL of CBR-TDR luciferase viral supernatant (collected in step 1.3) per well.
4. Centrifuge at 1,240 x g for 90 min at 32 °C.
Transduction
1. Count the T cells.
2. Aspirate the viral supernatant without scratching the bottom of the plate.
3. Plate two million T cells per well in 6 mL of Dulbecco's modified Eagle's medium (DMEM) containing 30 IU/mL human IL-2.
4. Examine the T cells daily. The T cells are ready to be expanded when they are nearly confluent, usually after 2 days.
5. When the cells are nearly confluent, gently wash them off the bottom of the plate using a pipette and transfer each well to a separate T75 flask. Add 9 mL of media for a total of 15 mL of media per flask.
6. The next day, add an additional 15 mL of media. The cells should be ready to inject into mice the day after this addition of media. Confirm successful transduction by performing flow cytometry (the luciferase construct contains a TD tomato fluorophore that is visible in the PE channel)¹⁶.

3. Engraftment of luciferase-transduced T cells in immunocompromised mice

Prepare and count the T cells for injection.
1. Remove the T cells from the flasks and count. The cells are ready to inject when they have expanded 20x-30x, usually by day 7 post-activation.
2. Centrifuge the T cells at 800 x g for 5 min. Resuspend in 2 mL of media and remove the beads using a magnet rack.
3. For experiments where T cells will be injected separately from bispecific antibodies, count the T cells and resuspend so that the final concentration is 20 million T cells per 100 µL of media. Skip to step 3.2. For experiments using ex vivo armed T cells (EATs), skip to step 3.1.4.
4. For experiments using ex vivo armed T cells, count the T cells and separate them into individual 1.5 mL tubes for each group, with 20 million cells per mouse. For example, if there are three groups of five mice each, prepare three 1.5 mL tubes with 100 million T cells each.
5. Centrifuge the 1.5 mL tubes at 800 x g for 5 min. Remove the media carefully without disturbing the T cell pellet. Resuspend in no more than 50 µL of media containing the bispecific antibodies. Incubate at RT for 30 min.
  NOTE: For the purposes of experiments conducted in this study, proprietary IgG-[L]-scFv T cell-engaging bispecific antibodies generated in the lab were used. For T cell arming, use 5 µg of antibody per 20 x 10⁶ T cells. Commercially available bispecific antibodies could also be used.
6. Wash away excess antibodies by adding 1,450 µL of media to each tube. Centrifuge at 800 x g for 5 min, carefully aspirate the media, and resuspend at a concentration of 20 million armed T cells per 100 µL media.
Injection and engraftment into mice
1. Anesthetize the mice in a chamber supplying 3.5% (v/v) inhaled isoflurane in 1 L/min oxygen. The mice are fully anesthetized when the hind limb pedal withdrawal reflex has disappeared.
  NOTE: Provide thermal support throughout the procedure.
2. Using a 26 G needle, inject 20 million T cells in 100 µL of media retroorbitally per mouse.
3. Administer 1,000 U recombinant IL-2 subcutaneously to support T cell survival in vivo.
4. Administer the bispecific antibodies retroorbitally (into the eye not used for T cell injection) or intraperitoneally. Allow the mice to recover from anesthesia and return to their cages.
  NOTE: Again, here, proprietary antibodies that were generated in the lab were used, but commercially available antibodies could be used instead. In the experiments here, 0.3-10 µg of antibody per mouse per dose was administered. The antibodies were administered twice per week for 3-4 weeks.

4. In vivo imaging of mice engrafted with luciferase-transduced T cells

NOTE: This step is to be performed on the day of imaging, which is not necessarily the same day that the T cells and/or antibodies are administered to the mice. Typically, we perform imaging 24 h after administration of the luciferase-transduced T cells.

Preparation of D-luciferin
1. Dissolve 1 g of D-luciferin in 33.3 mL of sterile PBS (final concentration: 30 mg/mL).
2. Aliquot the dissolved D-luciferin into 33 x 1.5 mL microcentrifuge tubes and keep the tubes at -20 °C.
3. On the day of imaging, thaw enough aliquots of 30 mg/mL D-luciferin for the number of animals to be imaged. One tube is enough for 10 animals.
  NOTE: Refreeze the remaining D-luciferin after use. D-luciferin is stable for at least five freeze/thaw cycles.
Administration of D-luciferin to mice
NOTE: Before administering D-luciferin to the mice, open the imaging software and initialize the system. The camera may take several minutes to cool, and this should be done before the mice are injected with D-luciferin to ensure that imaging can take place 5 min after administration of the substrate.
1. Anesthetize up to five mice in a chamber supplying 3.5% (v/v) inhaled isoflurane in 1 L/min oxygen. The mice are fully anesthetized when the hind limb pedal withdrawal reflex has disappeared.
2. Once the mice are fully anesthetized, administer 100 µL of 30 mg/mL D-luciferin per mouse (3 mg per mouse) by retroorbital injection with a 26 G needle. Image this group of mice before administering D-luciferin to the next group. Place the next group of mice in the isoflurane chamber to be anesthetized while the previous group is being imaged.
Imaging luciferase-transduced T cells
1. Move the anesthetized mice to the light-tight chamber of the imager and continue administering 3% isoflurane at 0.5 L/min. Place the mice on their sides such that the flank bearing the xenograft is facing up toward the camera. Take another set of images with the mice in a supine position to evaluate T cell presence in the lungs.
2. Using the Acquisition Control Panel, select Luminescent, Photograph, and Overlay. Set the exposure time to auto, the binning to medium, and F/Stop to 1. Acquire images. After the first image, set the exposure time to match that which was automatically calculated for the first image so that subsequent images may be compared directly. It may be useful to capture images with multiple exposure times to determine the optimal exposure time for achieving the brightest signal without pixel saturation.
3. Remove the mice from isoflurane, return to their cages, and observe until they are awake and ambulatory.
4. Repeat the steps from step 4.2.1 until all groups have been imaged.

Wyniki

As described in step 4.3, mice can be oriented in different positions during imaging to evaluate the presence of T cells in different tissues. Supine positioning allows for the assessment of T cells in the lungs, which is common at early time points after injection. Lateral positioning with the subcutaneous xenograft facing up is used to best assess T cell trafficking to the tumor. Female C.Cg-Rag2^tm1FwaIl2rg^tm1Sug/JicTac mice were used for all experiments described in this manuscript.

Dyskusje

While the T-BsAb blinatumomab has been approved for CD19-positive hematological malignancies, the successful implementation of T-BsAbs in solid tumors has proven much more difficult. Catumaxomab, a T-BsAb directed against epithelial cell adhesion molecule (EPCAM), was approved for the treatment of malignant ascites in ovarian cancer patients, but production of the drug was subsequently halted for commercial reasons¹⁹. No other T-BsAbs have been approved for solid tumors, underlining the challenges...

Ujawnienia

NKC reports receiving commercial research grants from Y-mAbs Therapeutics. NKC is the inventor and owner of issued patents licensed by MSK to Y-mAbs Therapeutics, Biotec Pharmacon/Lallemand, and Abpro-labs. MSK and NKC have financial interest in Y-mAbs. NKC reports receiving stock options from Eureka Therapeutics. HFG and MEC have no relevant disclosures.

Podziękowania

The authors would like to thank Dr. Vladimir Ponomarev for sharing the luciferase constructs used in the experiments described in the representative results section of this article.

Materiały

Name	Company	Catalog Number	Comments
293T cells	ATCC	CRL-11268
BSA	Sigma Aldrich	A7030-10G
CD3/CD28 beads	Gibco (ThermoFisher)	11161D
D-Luciferin, Potassium Salt	Goldbio	LUCK-1G
DMEM	Gibco (ThermoFisher)	11965092
DNA in vitro transfection reagent (polyjet)	SignaGen Laboratories	SL100688
EDTA	Sigma Aldrich	E9884-100G
FBS	Gibco (ThermoFisher)	10437028
Gag/pol plasmid	Addgene	14887
GFP plasmid	Addgene	11150-DNA.cg
Penicilin-Streptomycin	Gibco (ThermoFisher)	15140122
Recombinant human IL-2	R&D Systems	202-IL-010/CF
Retronectin	Takara	T100B
Trypsin	Gibco (ThermoFisher)	25-300-120
VSV-G plasmid	Addgene	8454

Odniesienia

Gökbuget, N., et al. Blinatumomab for minimal residual disease in adults with B-cell precursor acute lymphoblastic leukemia. Blood. 131 (14), 1522-1531 (2018).
Runcie, K., Budman, D. R., John, V., Seetharamu, N. Bi-specific and tri-specific antibodies- the next big thing in solid tumor therapeutics. Molecular Medicine. 24 (1), 50 (2018).
Dreier, T., et al. T Cell costimulus-independent and very efficacious inhibition of tumor growth in mice bearing subcutaneous or leukemic human B cell lymphoma xenografts by a CD19-/CD3- Bispecific single-chain antibody construct. The Journal of Immunology. 170 (8), 4397-4402 (2003).
Offner, S., Hofmeister, R., Romaniuk, A., Kufer, P., Baeuerle, P. A. Induction of regular cytolytic T cell synapses by bispecific single-chain antibody constructs on MHC class I-negative tumor cells. Molecular Immunology. 43 (6), 763-771 (2006).
Santich, B. H., Cheung, N. V., Klein, C. Editorial: Bispecific antibodies for T-cell based immunotherapy. Frontiers in Oncology. 10, 628005 (2020).
Santich, B. H., et al. Interdomain spacing and spatial configuration drive the potency of IgG-[L]-scFv T cell bispecific antibodies. Science Translational Medicine. 12 (534), eaax1315 (2020).
Wang, L., Hoseini, S. S., Xu, H., Ponomarev, V., Cheung, N. K. Silencing Fc domains in T cell-engaging bispecific antibodies improves T-cell trafficking and antitumor potency. Cancer Immunology Research. 7 (12), 2013-2024 (2019).
Park, J. A., Cheung, N. V. GD2 or HER2 targeting T cell engaging bispecific antibodies to treat osteosarcoma. Journal of Hematology & Oncology. 13 (1), 172 (2020).
Wu, Z., Guo, H. F., Xu, H., Cheung, N. V. Development of a tetravalent anti-GPA33/anti-CD3 bispecific antibody for colorectal cancers. Molecular Cancer Therapeutics. 17 (10), 2164-2175 (2018).
Lin, T. Y., Park, J. A., Long, A., Guo, H. F., Cheung, N. V. Novel potent anti-STEAP1 bispecific antibody to redirect T cells for cancer immunotherapy. Journal for Immunotherapy of Cancer. 9 (9), e003114 (2021).
Hoseini, S. S., Espinosa-Cotton, M., Guo, H. F., Cheung, N. V. Overcoming leukemia heterogeneity by combining T cell engaging bispecific antibodies. Journal for Immunotherapy of Cancer. 8 (2), e001626 (2020).
Hoseini, S. S., Guo, H., Wu, Z., Hatano, M. N., Cheung, N. V. A potent tetravalent T-cell-engaging bispecific antibody against CD33 in acute myeloid leukemia. Blood Advances. 2 (11), 1250-1258 (2018).
Hoseini, S. S., et al. T cell engaging bispecific antibodies targeting CD33 IgV and IgC domains for the treatment of acute myeloid leukemia. Journal for Immunotherapy of Cancer. 9 (5), e002509 (2021).
Li, H., Er Saw, P., Song, E. Challenges and strategies for next-generation bispecific antibody-based antitumor therapeutics. Cellular and Molecular Immunology. 17 (5), 451-461 (2020).
Rajabzadeh, A., Hamidieh, A. A., Rahbarizadeh, F. Spinoculation and retronectin highly enhance the gene transduction efficiency of Mucin-1-specific chimeric antigen receptor (CAR) in human primary T cells. BMC Molecular and Cell Biology. 22 (1), 57 (2021).
Kleeman, B., et al. A guide to choosing fluorescent protein combinations for flow cytometric analysis based on spectral overlap. Cytometry Part A. 93 (5), 556-562 (2018).
Park, J. A., Santich, B. H., Xu, H., Lum, L. G., Cheung, N. V. Potent ex vivo armed T cells using recombinant bispecific antibodies for adoptive immunotherapy with reduced cytokine release. Journal for Immunotherapy of Cancer. 9 (5), e002222 (2021).
Park, J. A., Wang, L., Cheung, N. V. Modulating tumor infiltrating myeloid cells to enhance bispecific antibody-driven T cell infiltration and anti-tumor response. Journal of Hematology & Oncology. 14 (1), 142 (2021).
Ströhlein, M. A., Heiss, M. M. The trifunctional antibody catumaxomab in treatment of malignant ascites and peritoneal carcinomatosis. Future Oncology. 6 (9), 1387-1394 (2010).
Rabinovich, B. A., et al. Visualizing fewer than 10 mouse T cells with an enhanced firefly luciferase in immunocompetent mouse models of cancer. Proceedings of the National Academy of Sciences. 105 (38), 14342-14346 (2008).
Skovgard, M. S., et al. Imaging CAR T-cell kinetics in solid tumors: Translational implications. Molecular Therapy Oncolytics. 22, 355-367 (2021).

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