Tracking Peripheral Blood Mononuclear Cells With Fluorine MRI

NCT ID: NCT02921373

Last Updated: 2024-07-24

Basic Information

• Recruitment Status: WITHDRAWN
• Clinical Phase: PHASE1
• Study Classification: INTERVENTIONAL
• Study Start Date: 2019-07-31
• Study Completion Date: 2022-12-31

Brief Summary

Cell-based therapies in the form of stem cell-based or immune cell-based therapies are becoming important treatment options that are either approved for clinical use or are showing promise in clinical trials. One of the issues regarding cell-based therapies is that, once the cells are injected into a subject, there is no easy way to track where they go, assess whether adequate numbers of cells arrive at the intended therapeutic target and for how long they persist at a given location. To address this issue non-invasive imaging methods have been developed using magnetic resonance imaging (MRI). When used with an appropriate cell labelling contrast agent, Cellular MRI can track cells non-invasively in vivo. Detection of cells is accomplished with an inert imaging agent containing the MRI sensitive fluorine-19 (19F) nuclei. The objective of this study is to demonstrate that 19F-MRI is safe to use in humans so that it can subsequently be used to track cell-based immunotherapies in future clinical trials. The long term goal is to be able to quantify immune cell migration to secondary lymphoid tissues and potentially to tumors and correlate to therapeutic outcomes.

Detailed Description

Background: None of the currently available Good Manufacturing Practices (GMP)-grade MRI cell labelling agents are approved for use in Canada. There is one iron oxide nanoparticle GMP grade preparation that is commercially available but it is not suitable for labelling the immune cell populations the investigators are interested in tracking in vivo. The investigators have, instead, chosen to develop the commercially available, GMP-grade 19F-based perfluorocarbon, known as Cell Sense, for the purpose of tracking immune cell-based vaccine therapies in vivo. This agent has been successful used in a phase I clinical trial in United States and is approved for a second trial current recruiting, under the oversight of the FDA.

The cell tracing agent Cell Sense (CS-1000) is an inert, non-metabolizable tracer. As CS-1000 is taken-up and incorporated into the cell traditional pharmacodynamic and pharmacokinetic analyses in animals and humans are not appropriate, as adsorption and biodistribution will vary with cell type, and therefore have not been done. In vitro studies of toxicity towards various cell types did not yield evidence of adverse effects on various cell functions. Cell Sense also was shown to be non-mutagenic using the Ames and Forward thymidine kinase (TK) assays. Some limited skin irritation was observed when >2,500 fold more Cell Sense than expected to be maximally injected into humans was injected intradermally into rats.

Examples of MRI cell tracking labels include superparamagnetic iron oxide nanoparticles and 19F-containing compounds such as perfluorocarbons. The advantage of using cellular MRI to track cells is that a non-radioactive tracer is used that is suitable for longitudinal studies. MRI offers 3D imaging with exquisite soft tissue contrast. The additional advantage of using 19F over iron-based agents is that 19F is a positive, easily quantifiable contrast cell labelling agent. Furthermore, there is no 19F-background MRI signal in humans whereas MRI involving iron can be confounded by different imaging artifacts and it is a negative contrast agent that is difficult to accurately quantify. The investigators are particularly interested in whether immune cells arrive in secondary lymphoid organs such as lymph nodes.

Study Design:

Open label, dose escalating, single centre, phase I study that will accrue (a) 6 healthy adults and (b) 6 prostate cancer patients.

Three healthy adults and three prostate cancer patients will be enrolled into the first cohort. Whole blood (150 ml) will be obtained by venipuncture. After processing of the blood to obtain peripheral blood mononuclear cells (PBMC), half of the PBMC will be treated with Cell Sense for 8-24 hours. Given the robustness of our data using 5 donors during dry runs, the investigators do not propose to compare labeled vs unlabeled cells as release criteria. However, the investigators will be collecting this data for information and research purposes. Three million (3 x 106) Cell Sense labeled autologous PBMC will be administered intradermally to the cohort 1 subjects. The three healthy adults and the 3 prostate cancer subjects will be tested concurrently.

If no grade 2 or higher adverse events are observed with the 1st cohort, concurrent enrolment will proceed to recruit a second set of 3 healthy adult subjects and the second set of 3 prostate cancer patients. The second cohort of subjects will be subjected to the same design but with an escalation of the dose to 2-3 x 107 Cell Sense-labeled autologous PBMC administered intradermally.

Endpoints:

Primary Endpoints:

Determine the feasibility of using Cell Sense to detect and monitor the migration of PBMC in humans

Secondary Endpoints:

• Confirm and further optimize the 19F Cell Sense detection and Hydrogen- 1 (1H) anatomical imaging parameters for imaging using the 19F/1H dual coil.
• Determine if Cell Sense-labeled PBMC migration to the draining lymph node can be detected.
• Determine if the lymph nodes in the area of interest imaged change in size on the injected side compared to the contralateral side.
• Quantify the number of Cell Sense-labeled PBMC detected.
• Evaluate safety parameters (toxicity) as defined by:
• adverse events.
• serious adverse events.
• changes in laboratory determination and vital sign parameters as assessed by medical history, physical examination and clinical laboratory tests.

The following categories will be used to grade any adverse events:

• Grade 1: does not interfere with daily activity,
• Grade 2: interferes with daily activity, no treatment required, except paracetamol,
• Grade 3: prevents daily activity or requires treatment.
• Grade 4: Life-threatening

NIH and FDA (or CTCAE v 4.0) guidelines will be used to determine the severity of adverse events

Conditions

Adverse Reaction to Diagnostic Agents and Kits Nos

Study Design

• Allocation Method: NON_RANDOMIZED
• Intervention Model: FACTORIAL
• Primary Study Purpose: BASIC_SCIENCE
• Blinding Strategy: NONE

Study Groups

Prostate Cancer Patients

Up to 6 Male prostate cancer patients with metastatic, castration resistant prostate cancer will be enrolled.

19F Cell Sense-labeled PBMC (3 million cells) will be injected intradermally into the upper thigh of each participant above the inguinal lymph node. MRI will be used to image the administration site.

Group Type: EXPERIMENTAL

19F Cell Sense-labeled PBMC

Intervention Type: BIOLOGICAL

Peripheral blood mononuclear cells (PBMC) will be isolated from patient whole blood samples and labeled in a GMP facility with GMP grade 19F Cell Sense imaging agent.

These cells will be re-administered to the patient prior to imaging.

MRI

Intervention Type: DEVICE

Participants will undergo Magnetic Resonance Imaging (MRI) at 1 hour and 24 hours following PBMC administration

Healthy Volunteers

Up to 6 male or female healthy volunteers will be enrolled.

19F Cell Sense-labeled PBMC (3 million cells) will be injected intradermally into the upper thigh of each participant above the inguinal lymph node. MRI will be used to image the administration site.

Group Type: EXPERIMENTAL

19F Cell Sense-labeled PBMC

Intervention Type: BIOLOGICAL

Peripheral blood mononuclear cells (PBMC) will be isolated from patient whole blood samples and labeled in a GMP facility with GMP grade 19F Cell Sense imaging agent.

These cells will be re-administered to the patient prior to imaging.

MRI

Intervention Type: DEVICE

Participants will undergo Magnetic Resonance Imaging (MRI) at 1 hour and 24 hours following PBMC administration

Interventions

19F Cell Sense-labeled PBMC

Peripheral blood mononuclear cells (PBMC) will be isolated from patient whole blood samples and labeled in a GMP facility with GMP grade 19F Cell Sense imaging agent.

These cells will be re-administered to the patient prior to imaging.

Intervention Type: BIOLOGICAL

MRI

Participants will undergo Magnetic Resonance Imaging (MRI) at 1 hour and 24 hours following PBMC administration

Intervention Type: DEVICE

Eligibility Criteria

Inclusion Criteria

• Men diagnosed with confirmed adenocarcinoma of the prostate
• No history of skin hypersensitivities or allergies.
• Normal liver functions as defined by alanine aminotransferase (ALT) (3-36 U/L) and aspirate aminotransferase (AST) levels (10-34 U/L)
• Normal kidney function by monitoring urea (2.5-8.0 ηmol/L) and creatine (70-120 μmol/L [for males]) concentrations.
• Normal complete blood count with differential
• Body Weight between 40 and 110 kg (relates to being able to fit in scanner)
• Body Mass Index < 30 (relates to being able to fit in scanner)
• Negative for (HIV, HTLV1&2, Hep A, B, C, syphilis) infection as determined by approved serological testing.

Exclusion Criteria

• Contraindication to venipuncture and donation of 100-160 mL of blood
• Active infection (not limited to HIV, HTLV1&2, Hep A, B, C, syphilis)
• Participants are on active chemotherapy (not including castrate hormone therapy), radiation therapy or immunosuppressive therapy (i.e. steroid use, anti-transplant rejection drugs, depleting antibodies)
• Participants who are unable to have an MRI scan (e.g. history of head or eye injury involving metal fragments, implanted electrical device (such as a cardiac pacemaker), conductive implants or devices such as skin patches, body piercing or tattoos containing metallic inks, severe heart disease (including susceptibility to heart rhythm abnormalities), claustrophobia, etc.)
• Participants with known allergies to phenol red, β-lactams and β-lactam derivative
• Participants with known allergies to streptomycin sulfate and gentamicin sulfate
• Participants with unforeseen conditions that are deemed unsafe or inappropriate for the study (e.g. participants who are claustrophobic and cannot undergo an MRI) as per the discretion of the principal investigator.

• Minimum Eligible Age: 40 Years
• Maximum Eligible Age: 85 Years
• Eligible Sex: ALL
• Accepts Healthy Volunteers: Yes

Sponsors

Western University, Canada

OTHER

Sponsor Role: collaborator

Ontario Institute for Cancer Research

OTHER

Sponsor Role: collaborator

Gregory A. Dekaban

OTHER

Sponsor Role: lead

Responsible Party

Gregory A. Dekaban

Professor

Responsibility Role: SPONSOR_INVESTIGATOR

Principal Investigators

Gregory A Dekaban, PhD

Role: PRINCIPAL_INVESTIGATOR

Robarts Research Institte - Western Universtiy

Paula J Foster, PhD

Role: PRINCIPAL_INVESTIGATOR

Robarts Research Institte - Western Universtiy

Sowmya Vuswanathan, PhD

Role: PRINCIPAL_INVESTIGATOR

University Health Network - University of Toronto

Joseph Chin, MD

Role: STUDY_CHAIR

London Health Research Institute - Western University

Michael Rieder, MD PhD

Role: STUDY_CHAIR

Robarts Research Institte - Western University

Gary Brahm, MD

Role: STUDY_CHAIR

London Health Research Institute

Doreen Matsui, MD

Role: STUDY_CHAIR

Western University

George Dresser, MD

Role: STUDY_CHAIR

Western University

Locations

Robarts Research Institute

London, Ontario, Canada

Countries

Canada

Other Identifiers

CS-PBMC-2015-001

Identifier Type: -

Identifier Source: org_study_id