#METABOLOMICS WORKBENCH cendalfr_20240411_073626 DATATRACK_ID:4770 STUDY_ID:ST003167 ANALYSIS_ID:AN005196 PROJECT_ID:PR001970 VERSION 1 CREATED_ON April 11, 2024, 8:12 am #PROJECT PR:PROJECT_TITLE Releasing the mitochondrial respiration brake MCJ/DnaJC15 enhances CD8 CAR-T PR:PROJECT_TITLE cell therapy efficacy PR:PROJECT_SUMMARY Metabolism of chimeric antigen receptor (CAR) T cells is emerging as an PR:PROJECT_SUMMARY important area to improve CAR-T cell therapy in cancer treatment. Mitochondrial PR:PROJECT_SUMMARY respiration is essential for survival and function of CAR-T cells, but PR:PROJECT_SUMMARY developing strategies to specifically enhance mitochondrial respiration has been PR:PROJECT_SUMMARY challenging. Here we identify MCJ/DnaJC15, an endogenous negative regulator of PR:PROJECT_SUMMARY mitochondrial Complex I, as a metabolic target to enhance mitochondrial PR:PROJECT_SUMMARY respiration in CD8 CAR-T cells. Loss of MCJ in CD8 CAR-T cells increases their PR:PROJECT_SUMMARY in vitro and in vivo efficacy against mouse B cell leukemias. MCJ deficiency in PR:PROJECT_SUMMARY TCR- specific CD8 cells also increases their efficacy against solid tumors in PR:PROJECT_SUMMARY vivo. Furthermore, we reveal that human CD8 cells express MCJ and that silencing PR:PROJECT_SUMMARY MCJ expression increases mitochondrial metabolism and anti-tumor activity of PR:PROJECT_SUMMARY human CAR-T cells. Thus, targeting MCJ to enhance mitochondrial metabolism is a PR:PROJECT_SUMMARY promising therapeutic strategy to improve the efficacy of adoptive T cell PR:PROJECT_SUMMARY therapies. PR:INSTITUTE University of Colorado School of Medicine PR:LABORATORY Laboratory of Angelo D'Alessandro in collaboration with Mercedes Rincon PR:LAST_NAME Cendali PR:FIRST_NAME Francesca PR:ADDRESS 13199 East Montview Boulevard, Aurora, CO, 80045, USA PR:EMAIL francesca.cendali@cuanschutz.edu PR:PHONE 3037246131 #STUDY ST:STUDY_TITLE Releasing the mitochondrial respiration brake MCJ/DnaJC15 enhances CD8 CAR-T ST:STUDY_TITLE cell therapy efficacy ST:STUDY_SUMMARY Metabolism of chimeric antigen receptor (CAR) T cells is emerging as an ST:STUDY_SUMMARY important area to improve CAR-T cell therapy in cancer treatment. Mitochondrial ST:STUDY_SUMMARY respiration is essential for survival and function of CAR-T cells, but ST:STUDY_SUMMARY developing strategies to specifically enhance mitochondrial respiration has been ST:STUDY_SUMMARY challenging. Here we identify MCJ/DnaJC15, an endogenous negative regulator of ST:STUDY_SUMMARY mitochondrial Complex I, as a metabolic target to enhance mitochondrial ST:STUDY_SUMMARY respiration in CD8 CAR-T cells. Loss of MCJ in CD8 CAR-T cells increases their ST:STUDY_SUMMARY in vitro and in vivo efficacy against mouse B cell leukemias. MCJ deficiency in ST:STUDY_SUMMARY TCR- specific CD8 cells also increases their efficacy against solid tumors in ST:STUDY_SUMMARY vivo. Furthermore, we reveal that human CD8 cells express MCJ and that silencing ST:STUDY_SUMMARY MCJ expression increases mitochondrial metabolism and anti-tumor activity of ST:STUDY_SUMMARY human CAR-T cells. Thus, targeting MCJ to enhance mitochondrial metabolism is a ST:STUDY_SUMMARY promising therapeutic strategy to improve the efficacy of adoptive T cell ST:STUDY_SUMMARY therapies. ST:INSTITUTE University of Colorado School of Medicine ST:LABORATORY Laboratory of Angelo D'Alessandro in collaboration with Mercedes Rincon ST:LAST_NAME Cendali ST:FIRST_NAME Francesca ST:ADDRESS 13199 East Montview Boulevard, Aurora, CO, 80045, USA ST:EMAIL francesca.cendali@cuanschutz.edu ST:PHONE 3037246131 #SUBJECT SU:SUBJECT_TYPE Cultured cells SU:SUBJECT_SPECIES Homo sapiens #SUBJECT_SAMPLE_FACTORS: SUBJECT(optional)[tab]SAMPLE[tab]FACTORS(NAME:VALUE pairs separated by |)[tab]Raw file names and additional sample data SUBJECT_SAMPLE_FACTORS - D16 19BBz_2 Factor:low 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=2 SUBJECT_SAMPLE_FACTORS - D16 19BBz_3 Factor:low 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=3 SUBJECT_SAMPLE_FACTORS - D16 19BBz_4 Factor:low 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=4 SUBJECT_SAMPLE_FACTORS - D26 19BBz_2 Factor:high 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=11 SUBJECT_SAMPLE_FACTORS - D26 19BBz_3 Factor:high 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=12 SUBJECT_SAMPLE_FACTORS - D26 19BBz_4 Factor:high 19BBz | Sample source:Cells RAW_FILE_NAME(Raw File)=13 #COLLECTION CO:COLLECTION_SUMMARY Human CD8 cells were isolated with positive selection as described. The CD8 CO:COLLECTION_SUMMARY cells were activated with anti-CD3/anti-CD28 beads (Dynabeads™ Human CO:COLLECTION_SUMMARY T-Expander CD3/CD28, Gibco), as previously described107. After 48h activation, CO:COLLECTION_SUMMARY the CD8 cells were spun (1000xg for 2h at 32C) with lentiviral supernatant CO:COLLECTION_SUMMARY containing CD19-BBz/shMCJ-1 CAR, CD19-BBz/shMCJ-2 CAR or CD19-BBz/shMCJ-2 CAR CO:COLLECTION_SUMMARY construct-packing virus with rhIL-2 (40 IU/ml) and protamine sulfate. After CO:COLLECTION_SUMMARY transduction, the anti-CD3/anti-CD28 beads were removed and CD8 cells were CO:COLLECTION_SUMMARY expanded with rhIL-2 (100 IU/ml) for the specified number of days. CO:SAMPLE_TYPE T-cells #TREATMENT TR:TREATMENT_SUMMARY The human CD19-BBz shRNA CAR lentiviral constructs were based on a previously TR:TREATMENT_SUMMARY described CD19-BBz CAR containing the human CD19-binding scFV FMC63, CD8 hinge TR:TREATMENT_SUMMARY domain, 4-1BB costimulatory domain and CD3 chain105. Using CD19-BBz CAR TR:TREATMENT_SUMMARY plasmid as a cloning vector, we generated multiple vectors where we incorporated TR:TREATMENT_SUMMARY the RNA polymerase III U6 promotor (on the 3' of the CD3 chain domain) TR:TREATMENT_SUMMARY followed by an shRNA: 1) a CD19-BBz/shMCJ-1 CAR construct containing the shMCJ-1 TR:TREATMENT_SUMMARY 5’-GAAGATTTCAACTCCTAGC-3’ sequence106, 2) a CD19-BBz/shMCJ-2 CAR construct TR:TREATMENT_SUMMARY containing the shMCJ-2; 5’-AACCTCTAGAACAAGTTATC-3’, and 3) a TR:TREATMENT_SUMMARY CD19-BBz/c-shRNA CAR vectors expressing the shRNA encoding scramble sequences. TR:TREATMENT_SUMMARY Lentiviral supernatant was produced in the LentiX-293T packaging cell line TR:TREATMENT_SUMMARY (Clonetech) as previously described. Lentiviral supernatants were collected TR:TREATMENT_SUMMARY after 48 hours post-transfection. #SAMPLEPREP SP:SAMPLEPREP_SUMMARY CAR-T cells were isolated as described above either from in vitro culture or SP:SAMPLEPREP_SUMMARY from bone marrow harvested in an in vivo study. The cells were washed in PBS and SP:SAMPLEPREP_SUMMARY frozen at -80C until the assay is ready to run. Metabolites from cells were SP:SAMPLEPREP_SUMMARY extracted at 2x106 cells/ml at 4°C (30 min) in the presence of 5:3:2 SP:SAMPLEPREP_SUMMARY MeOH:MeCN:water (v/v/v). The samples were spun down and the resulting SP:SAMPLEPREP_SUMMARY supernatant was transferred to new tubes and dried under a vacuum. The resulting SP:SAMPLEPREP_SUMMARY residue was reconstituted in 0.1% formic acid at a 3x concentration, then SP:SAMPLEPREP_SUMMARY analyzed on a Thermo Vanquish UHPLC coupled to a Thermo Q Exactive MS as SP:SAMPLEPREP_SUMMARY previously described in detail. #CHROMATOGRAPHY CH:CHROMATOGRAPHY_SUMMARY Negative ion Mode CH:CHROMATOGRAPHY_TYPE Reversed phase CH:INSTRUMENT_NAME Thermo Vanquish CH:COLUMN_NAME Phenomenex Kinetex C18 (30 x 2.1mm, 1.7um) CH:SOLVENT_A 100% Water; 10mM Ammonium acetate, .01% Formic Acid CH:SOLVENT_B 50% Methanol/ 50% Acetonitrile; 10mM Ammonium acetate, .01% Formic Acid CH:FLOW_GRADIENT 0-0.2 min 5% B, 0.2-.8 min hold at 95% B, .8-.81 min 95-5% B, .81-1 min hold at CH:FLOW_GRADIENT 5% B. CH:FLOW_RATE 0.450ml/min CH:COLUMN_TEMPERATURE 45 #ANALYSIS AN:ANALYSIS_TYPE MS #MS MS:INSTRUMENT_NAME Thermo Q Exactive Orbitrap MS:INSTRUMENT_TYPE Exploris120 MS:MS_TYPE ESI MS:ION_MODE NEGATIVE MS:MS_COMMENTS Resolution 70,000, scan range 65-900 m/z, maximum injection time 200 ms, MS:MS_COMMENTS microscans 2, automatic gain control (AGC) 3 x 10^6 ions, source voltage 4.0 kV, MS:MS_COMMENTS capillary temperature 320 C, and sheath gas 45, auxiliary gas 15, and sweep gas MS:MS_COMMENTS 0 (all nitrogen). Data converted to mzXML using RawConverter. Metabolites were MS:MS_COMMENTS annotated and integrated using Maven in conjunction with the KEGG database. #MS_METABOLITE_DATA MS_METABOLITE_DATA:UNITS Peak Areas MS_METABOLITE_DATA_START Samples D16 19BBz_1 D16 19BBz_2 D16 19BBz_3 D26 19BBz_2 D26 19BBz_3 D26 19BBz_4 Factors Factor:low 19BBz | Sample source:Cells Factor:low 19BBz | Sample source:Cells Factor:high 19BBz | Sample source:Cells Factor:high 19BBz | Sample source:Cells Factor:high 19BBz | Sample source:Cells ATP 19014.66 26227.63 16447.19 2206.066 1390.958 2917.118 Phosphate 21833840 22965410 23621400 21054690 18596380 20222680 Diphosphate 3173455 3622059 3854649 3952140 3478727 2549453 D-Glucose 351309.9 433952.1 325824.6 369659.3 306164.4 312890.2 D-Fructose 1-6-bisphosphate 146827.2 259145.7 228674.7 12428.3 17114.98 24310.78 D-Glyceraldehyde 3-phosphate/Glycerone phosphate 930077.3 690660.1 558928 976922.1 1457511 735174.5 2/3-Phospho-D-glycerate 60150.83 46892.61 80066.84 381.0097 502.2223 12902.58 Phosphoenolpyruvate 4157.771 8876.774 15065.4 0 0 2800.342 Pyruvate 84402.01 133531.6 90980.66 234081.5 210604.5 95224.38 Lactate 4611334 7797466 7531226 7079256 6972118 3402812 Mannitol 42364.34 82909.54 109113.8 153467.3 187324.9 48378.62 Citrate 141050.3 176027.1 157177 98102.71 146129.8 99637.65 2-Oxoglutarate 8487.82 12050.6 6578.336 1287.222 2813.854 3613.314 Succinate 49954.75 84106.76 74866.57 112383 107117.8 44798.08 Fumarate 72002.36 60629.3 46702.17 13292.89 17005.37 24117.62 Malate 452675.2 403095.8 306856.8 76249.38 109483.5 166152.3 4-Acetamidobutanoate 4583.899 7702.877 8920.666 17016.33 18558.4 3859.461 Octanoic acid (caprylate) 2993856 4182712 1153829 4866070 5023588 1946367 Nonanoic acid (pelargonate) 109969.9 117714.5 81422.14 112241.5 123672.1 74494.55 Decanoic acid (caprate) 45847.74 55780.47 42193.36 59552.89 65901.07 39853.85 Dodecanoic acid 12245.82 17391.16 14257.24 10060.08 13218.41 8528.238 Tetradecanoic acid 17870.01 18869.06 16064.83 20769.71 20445.1 14913.76 Hexadecanoic acid 600047.1 638391.4 517900.9 1131847 765317 512133.7 Hexadecenoic acid 31826.61 26635.73 33079.71 21976.22 25815.62 20764.3 Octadecenoic acid 151570.7 157885.7 134179.4 157201.1 132413.5 99215.78 Linoleate 20670.14 33157.76 22990.34 24674.27 30690.86 8576.772 Dodecanedioic acid 2239.513 2909.635 4659.193 3219.257 6314.243 3302.674 MS_METABOLITE_DATA_END #METABOLITES METABOLITES_START metabolite_name CmpdID parent medRt ATP C00002 505.9875 0.3576738 Phosphate C00009 96.96812 0.2040902 Diphosphate C00013 176.9349 0.18636 D-Glucose C00031 179.0552 0.2114511 D-Fructose 1-6-bisphosphate C00354 338.9886 0.1983463 D-Glyceraldehyde 3-phosphate/Glycerone phosphate C00118 168.9883 0.5055173 2/3-Phospho-D-glycerate C00631 184.9847 0.2106258 Phosphoenolpyruvate C00074 166.974 0.2086936 Pyruvate C00022 87.00727 0.2537393 Lactate C01432 89.0229 0.2570731 Mannitol C00392 181.0704 0.2702953 Citrate C00158 191.0189 0.2063361 2-Oxoglutarate C00026 145.013 0.2116728 Succinate C00042 117.0179 0.2344009 Fumarate C00122 115.0023 0.2281322 Malate C00149 133.0129 0.1987566 4-Acetamidobutanoate C02946 144.0654 0.2938338 Octanoic acid (caprylate) C06423 143.1065 0.5209751 Nonanoic acid (pelargonate) C01601 157.1223 0.5523673 Decanoic acid (caprate) C01571 171.138 0.5745994 Dodecanoic acid C02679 199.1696 0.6075237 Tetradecanoic acid C06424 227.2011 0.6438132 Hexadecanoic acid C00249 255.2327 0.6944952 Hexadecenoic acid C08362 253.2171 0.6539506 Octadecenoic acid C00712 281.2485 0.7043023 Linoleate C01595 279.2329 0.665722 Dodecanedioic acid C02678 229.144 0.4839389 METABOLITES_END #END