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Autologous Mobilized Peripheral Blood CD34+ Hematopoietic Stem and Progenitor Cells (HSPC) Transduced With the Elongation Factor Alpha Short Promoter (EFS) - Adenosine Deaminase (ADA) Gene (EFS-ADA) Lentiviral Vector for Adenosine Deaminase Severe Combined Immune Deficiency (ADA SCID)

Primary Purpose

Adenosine Deaminase Severe Combined Immune Deficiency

Status
Recruiting
Phase
Phase 1
Locations
United States
Study Type
Interventional
Intervention
A cryopreserved formulation of autologous mPB CD34+ hematopoietic stem and progenitor cells transduced ex vivo with the EFS-ADA lentiviral vector encoding the human ADA enzyme
Sponsored by
University of California, Los Angeles
About
Eligibility
Locations
Arms
Outcomes
Full info

About this trial

This is an interventional treatment trial for Adenosine Deaminase Severe Combined Immune Deficiency focused on measuring Gene Therapy, Hematopoietic Stem Cell, Lentiviral Vector, Reduced Intensity Conditioning with Busulfan

Eligibility Criteria

1 Month - undefined (Child, Adult, Older Adult)All SexesDoes not accept healthy volunteers

Inclusion Criteria:

All subjects must fulfill the following criteria to be included in the study:

  1. Provision of written informed consent prior to any study related procedures. In this study consent must be provided by the parents/legal guardians and, where applicable according to local laws, a signed assent from the child,
  2. Subjects ≥30 days of age,
  3. With a diagnosis of ADA-SCID based on:

    Evidence of ADA deficiency, defined as:

    i. Decreased ADA enzymatic activity in erythrocytes, leukocytes, skin fibroblasts, or in cultured fetal cells to levels consistent with ADA-SCID as determined by the reference laboratory, or ii. Identified mutations in ADA alleles consistent with a severe reduction in ADA activity,

    Evidence of ADA-SCID based on either:

    i. Family history of a first order relative with ADA deficiency and clinical and laboratory evidence of severe immunologic deficiency, or ii. Evidence of severe immunologic deficiency in subjects prior to the institution of immune restorative therapy, based on

    1. Lymphopenia (absolute lymphocyte count (ALC) <400 cells/mL) OR absence or low number of T cells (absolute CD3+ count < 300 cells/mL), or
    2. Severely decreased T lymphocyte blastogenic responses to phytohemagglutinin (either <10% of lower limit of normal controls for the diagnostic laboratory, or <10% of the response of the normal control of the day, or stimulation index <10), or
    3. Identification of SCID by neonatal screening revealing low T Cell Receptor Excision Circles (TREC) levels.
  4. Ineligible for matched family allogeneic bone marrow (BM) transplantation, defined as the absence of a medically eligible HLA-identical sibling or family donor, with normal immune function, who could serve as an allogeneic bone marrow donor.
  5. Females of child-bearing age will be required to provide a negative pregnancy test 30 days prior to Visit 2.
  6. Subjects and their parents/legal guardians must be willing and able to comply with study restrictions and to remain at the clinic for the required duration during the study period and willing to return to the clinic for the follow up evaluation as specified in the protocol.

Exclusion Criteria:

Subjects will not be eligible for the study if any of the following criteria is fulfilled:

  1. Ineligible for autologous HSCT as per clinical site criteria
  2. Other conditions which in the opinion of the Principal Investigator and/or Co Investigators, contraindicate the mobilization of peripheral blood or the leukapheresis process, the administration of busulfan and the infusion of transduced cells, or which indicate an inability of the subject or subject's parent/legal guardian to comply with the protocol
  3. Hematologic abnormality, defined as:

    • Anemia (Hb <8.0 g/dl).
    • Neutropenia (ANC <500/mm3). Note: ANC <500 with absence of myelodysplastic syndrome on bone marrow aspirate and biopsy and normal marrow cytogenetics are acceptable for eligibility.
    • Thrombocytopenia (platelet count <50,000/mm3, at any age).
    • Prothrombin time or international normalized ratio (INR) and partial thromboplastin time (PTT) >2 x upper limit of normal (ULN) (subjects with a correctable deficiency controlled on medication will not be excluded).
    • Cytogenetic abnormalities on peripheral blood or bone marrow or amniotic fluid (if available).
    • Prior allogeneic HSCT with cytoreductive conditioning.
  4. Pulmonary abnormality, defined as:

    • Resting O2 saturation by pulse oximetry <90% on room air.
    • Chest X-ray indicating active or progressive pulmonary disease. Note: Chest X ray indicating residual signs of treated pneumonitis is acceptable for eligibility.
  5. Cardiac abnormality, defined as:

    • Abnormal ECG indicating cardiac pathology.
    • Uncorrected congenital cardiac malformation with clinical symptoms.
    • Active cardiac disease, including clinical evidence of congestive heart failure, cyanosis, hypotension.
    • Poor cardiac function as evidenced by left ventricular ejection fraction <40% on echocardiogram.
  6. Neurologic abnormality, defined as:

    • Significant neurologic abnormality revealed by examination.
    • Uncontrolled seizure disorder.
  7. Renal abnormality, defined as:

    • Renal insufficiency: serum creatinine ≥1.2 mg/dl (106 µmol/L), or ≥3+ proteinuria.
    • Abnormal serum sodium, potassium, calcium, magnesium or phosphate levels at >2 x ULN.
  8. Hepatic/gastrointestinal abnormality, defined as:

    • Serum transaminases >5 x ULN.
    • Serum bilirubin >2 x ULN.
    • Serum glucose >1.5 x ULN.
  9. Oncologic disease, defined as:

    • Evidence of active malignant disease other than dermatofibrosarcoma protuberans (DFSP).
    • Evidence of DFSP expected to require anti-neoplastic therapy within the 5 years following the infusion of genetically corrected cells (if anti-neoplastic therapy has been completed, a subject with a history of DFSP can be included).
    • Evidence of DFSP expected to be life limiting within the 5 years following the infusion of genetically corrected cells.
  10. Known sensitivity to Busulfan.
  11. Confirmation of an infectious disease by deoxyribonucleic acid (DNA) polymerase chain reaction (PCR) positive at time of assessment for the following:

    • HIV-1,
    • Hepatitis B,
    • Parvovirus B19.
  12. The subject is pregnant or has a major congenital anomaly.
  13. Is likely to require treatment during the study with drugs that are not permitted by the study protocol.
  14. The subject has previously received another form of gene therapy.

Sites / Locations

  • University of California, Los Angeles (UCLA)Recruiting

Arms of the Study

Arm 1

Arm Type

Experimental

Arm Label

Autologous mobilized peripheral blood (mPB) transduced with EFS ADA lentiviral vector

Arm Description

Evaluate safety and efficacy of this autologous gene therapy

Outcomes

Primary Outcome Measures

Survival
The primary study outcome will be to determine survival for all subjects 2 years after gene therapy

Secondary Outcome Measures

Evaluate Safety from clinical adverse events.
Evaluate safety of the treatment by recording clinical adverse events (AE).
Evaluate Safety from replication competent lentivirus by quantitative polymerase chain reaction (qPCR) assay.
Evaluate safety by recording incidents of replication competent lentivirus by qPCR assay..
Evaluate Safety from vector-related clonal expansion by non-restrictive Linear Amplification Polymerase Chain Reaction (nrLAM-PCR)
Evaluate safety by recording incidence of vector-related clonal expansion by nrLAM-PCR
Record event free survival at 24 months
Record Event Free Survival as a definition of "failure" of the therapy. Event-free survival is defined as the proportion of subjects alive with no "event", an "event" being the resumption of PEG-ADA ERT or the need for a rescue allogeneic hematopoietic stem cell transplant (HSCT), or death.
Determine incidence of Infection over two years after gene therapy
Determine the incidence and severity of infections post-gene therapy (subsequent to hematopoietic reconstitution). Over 2 years, record the incidence of hospitalizations or outpatient-based treatments for systemic bacterial, fungal, or viral infections (including, but not limited to Cytomegalovirus (CMV) infections).
Neuro-developmental Outcomes by neurodevelopmental testing (subjects 5-7 yeas of age)
Measure neuro-developmental status post-gene therapy. Perform age-appropriate neuro-developmental assessments testing (5- 7 years of age) at baseline and 2 years post-gene therapy - Wechsler Scale of Intelligence
Neuro-developmental Outcomes by neurodevelopmental testing (subjects 1 year -42 month of age)
Measure neuro-developmental status post-gene therapy. Perform age-appropriate neuro-developmental assessments testing (1 year to 42 months of age) at baseline and 2 years post-gene therapy - : Bayley Scale of Infant Development
Neuro-developmental Outcomes by Brain Stem Evoked Response (BAER) testing
Measure neuro-developmental status post-gene therapy - Perform Brainstem Auditory Evoked Response test at baseline and at 2 years.
Cessation of immunoglobulin replacement therapy (IgRT).
Record time post-gene therapy that immunoglobulin replacement therapy (IgRT) is stopped based on defined criteria.

Full Information

First Posted
June 4, 2022
Last Updated
January 24, 2023
Sponsor
University of California, Los Angeles
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1. Study Identification

Unique Protocol Identification Number
NCT05432310
Brief Title
Autologous Mobilized Peripheral Blood CD34+ Hematopoietic Stem and Progenitor Cells (HSPC) Transduced With the Elongation Factor Alpha Short Promoter (EFS) - Adenosine Deaminase (ADA) Gene (EFS-ADA) Lentiviral Vector for Adenosine Deaminase Severe Combined Immune Deficiency (ADA SCID)
Official Title
Efficacy and Safety of Cryopreserved Autologous Mobilized Peripheral Blood CD34+ Hematopoietic Stem and Progenitor Cells Transduced Ex Vivo With the EFS-ADA Lentiviral Vector in Patients With Severe Combined Immune Deficiency Due To Adenosine Deaminase Deficiency
Study Type
Interventional

2. Study Status

Record Verification Date
January 2023
Overall Recruitment Status
Recruiting
Study Start Date
January 4, 2023 (Actual)
Primary Completion Date
December 2024 (Anticipated)
Study Completion Date
December 2024 (Anticipated)

3. Sponsor/Collaborators

Responsible Party, by Official Title
Principal Investigator
Name of the Sponsor
University of California, Los Angeles

4. Oversight

Studies a U.S. FDA-regulated Drug Product
Yes
Studies a U.S. FDA-regulated Device Product
No
Data Monitoring Committee
Yes

5. Study Description

Brief Summary
The aim of this study is to assess the safety and efficacy of autologous transplantation of hematopoietic stem cells (CD34+ cells) from mobilized peripheral blood (mPB) of ADA-deficient SCID infants and children following human ADA gene transfer by the EFS-ADA lentiviral vector. The level of gene transfer in blood cells and immune function will be measured as endpoints.
Detailed Description
The study is open to twenty (20) infants and children diagnosed with ADA-deficient SCID who did not have a medically eligible, human leukocyte antigen (HLA)-identical sibling donor for bone marrow transplantation. The EFS-ADA lentiviral vector with the human ADA complementary DNA (cDNA) will be used to transduce autologous CD34+ cells from Granulocyte Colony Stimulating Factor (G-CSF)/Plerixafor mobilized Peripheral Blood (mPB) of these subjects. The subjects will receive pharmacokinetically-adjusted busulfan reduced intensity conditioning prior to re-infusion of their gene-modified cells. Overall survival at two years is the primary endpoint. During the follow-up phase, the investigators aim to determine whether the cells could engraft and produce mature cells that contain and express the corrected ADA gene in the absence of pegylated adenosine deaminase (PEG-ADA) enzyme replacement therapy (ERT), which will be withheld starting on Day +30 following transplant. Efficacy studies to evaluate the level of immune reconstitution, will be performed in the two years of the study. Patients will be asked to enroll into a long-term follow-up study to reach a total of 15 years follow-up after gene therapy.

6. Conditions and Keywords

Primary Disease or Condition Being Studied in the Trial, or the Focus of the Study
Adenosine Deaminase Severe Combined Immune Deficiency
Keywords
Gene Therapy, Hematopoietic Stem Cell, Lentiviral Vector, Reduced Intensity Conditioning with Busulfan

7. Study Design

Primary Purpose
Treatment
Study Phase
Phase 1, Phase 2
Interventional Study Model
Single Group Assignment
Model Description
Prospective, non-randomized Phase I/II clinical trial to assess the safety and efficacy of gene therapy for ADA SCID by transplantation of autologous mPB CD34+ hematopoietic stem and progenitor cells (HSPC) transduced by the EFS-ADA lentiviral vector.
Masking
None (Open Label)
Allocation
N/A
Enrollment
20 (Anticipated)

8. Arms, Groups, and Interventions

Arm Title
Autologous mobilized peripheral blood (mPB) transduced with EFS ADA lentiviral vector
Arm Type
Experimental
Arm Description
Evaluate safety and efficacy of this autologous gene therapy
Intervention Type
Combination Product
Intervention Name(s)
A cryopreserved formulation of autologous mPB CD34+ hematopoietic stem and progenitor cells transduced ex vivo with the EFS-ADA lentiviral vector encoding the human ADA enzyme
Intervention Description
Autologous transplantation of EFS-ADA lentiviral vector transduced, mPB CD34+ cells by central venous infusion, following reduced intensity conditioning with busulfan
Primary Outcome Measure Information:
Title
Survival
Description
The primary study outcome will be to determine survival for all subjects 2 years after gene therapy
Time Frame
24 months
Secondary Outcome Measure Information:
Title
Evaluate Safety from clinical adverse events.
Description
Evaluate safety of the treatment by recording clinical adverse events (AE).
Time Frame
24 months
Title
Evaluate Safety from replication competent lentivirus by quantitative polymerase chain reaction (qPCR) assay.
Description
Evaluate safety by recording incidents of replication competent lentivirus by qPCR assay..
Time Frame
24 months
Title
Evaluate Safety from vector-related clonal expansion by non-restrictive Linear Amplification Polymerase Chain Reaction (nrLAM-PCR)
Description
Evaluate safety by recording incidence of vector-related clonal expansion by nrLAM-PCR
Time Frame
24 months
Title
Record event free survival at 24 months
Description
Record Event Free Survival as a definition of "failure" of the therapy. Event-free survival is defined as the proportion of subjects alive with no "event", an "event" being the resumption of PEG-ADA ERT or the need for a rescue allogeneic hematopoietic stem cell transplant (HSCT), or death.
Time Frame
24 months
Title
Determine incidence of Infection over two years after gene therapy
Description
Determine the incidence and severity of infections post-gene therapy (subsequent to hematopoietic reconstitution). Over 2 years, record the incidence of hospitalizations or outpatient-based treatments for systemic bacterial, fungal, or viral infections (including, but not limited to Cytomegalovirus (CMV) infections).
Time Frame
24 months
Title
Neuro-developmental Outcomes by neurodevelopmental testing (subjects 5-7 yeas of age)
Description
Measure neuro-developmental status post-gene therapy. Perform age-appropriate neuro-developmental assessments testing (5- 7 years of age) at baseline and 2 years post-gene therapy - Wechsler Scale of Intelligence
Time Frame
24 months
Title
Neuro-developmental Outcomes by neurodevelopmental testing (subjects 1 year -42 month of age)
Description
Measure neuro-developmental status post-gene therapy. Perform age-appropriate neuro-developmental assessments testing (1 year to 42 months of age) at baseline and 2 years post-gene therapy - : Bayley Scale of Infant Development
Time Frame
24 months
Title
Neuro-developmental Outcomes by Brain Stem Evoked Response (BAER) testing
Description
Measure neuro-developmental status post-gene therapy - Perform Brainstem Auditory Evoked Response test at baseline and at 2 years.
Time Frame
24 months
Title
Cessation of immunoglobulin replacement therapy (IgRT).
Description
Record time post-gene therapy that immunoglobulin replacement therapy (IgRT) is stopped based on defined criteria.
Time Frame
24 months
Other Pre-specified Outcome Measures:
Title
Exploratory Study Objectives to measure biological correlates of efficacy - Vector Copy Number (VCN) in peripheral blood leukocytes
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 1. Quantify gene marking by vector copy number (VCN) in peripheral blood leukocytes by droplet digital polymerase chain reaction (ddPCR).
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy (Vector integrant diversity)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 2. Quantify clonal diversity of vector integrants by non-restrictive Linear Amplification polymerase chain reaction (nrLAM-PCR). nrLAM-PCR identifies all distinct vector integrants in a cell sample from patients. The presence of >1,000 unique integration sites in a sample indicates diversity of hematopoietic stem cell of clonal engraftment
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy (expressed ADA enzyme in erythrocytes)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 3. Measure ADA enzyme activity in erythrocytes as an indicator of expression of functional ADA enzyme from the vector.
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy Deoxyadenosine nucleotides in erythrocytes)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 4. Measure total deoxyadenosine nucleotides in erythrocytes.
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy (Immune reconstitution - quantify T and B cell)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 5. Assess immune reconstitution by measuring absolute numbers of T and B cells .
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy (Immune reconstitution - measure serum immunoglobulins)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 6. Assess immune reconstitution by measuring serum immunoglobulin levels
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy (Immune reconstitution - response to tetanus vaccine)
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 7. Assess immune reconstitution by measuring response to tetanus vaccine by measuring serum anti-tetanus antibody titers after tetanus vaccination
Time Frame
24 months
Title
Exploratory Study Objectives to measure biological correlates of efficacy Parent report Quality of Life
Description
The Exploratory Study Objectives are to measure biological correlates of efficacy. 8. Parent-Reported Quality of Life (PedsQL 4.0) at baseline and 2 years.
Time Frame
24 months

10. Eligibility

Sex
All
Minimum Age & Unit of Time
1 Month
Accepts Healthy Volunteers
No
Eligibility Criteria
Inclusion Criteria: All subjects must fulfill the following criteria to be included in the study: Provision of written informed consent prior to any study related procedures. In this study consent must be provided by the parents/legal guardians and, where applicable according to local laws, a signed assent from the child, Subjects ≥30 days of age, With a diagnosis of ADA-SCID based on: Evidence of ADA deficiency, defined as: i. Decreased ADA enzymatic activity in erythrocytes, leukocytes, skin fibroblasts, or in cultured fetal cells to levels consistent with ADA-SCID as determined by the reference laboratory, or ii. Identified mutations in ADA alleles consistent with a severe reduction in ADA activity, Evidence of ADA-SCID based on either: i. Family history of a first order relative with ADA deficiency and clinical and laboratory evidence of severe immunologic deficiency, or ii. Evidence of severe immunologic deficiency in subjects prior to the institution of immune restorative therapy, based on Lymphopenia (absolute lymphocyte count (ALC) <400 cells/mL) OR absence or low number of T cells (absolute CD3+ count < 300 cells/mL), or Severely decreased T lymphocyte blastogenic responses to phytohemagglutinin (either <10% of lower limit of normal controls for the diagnostic laboratory, or <10% of the response of the normal control of the day, or stimulation index <10), or Identification of SCID by neonatal screening revealing low T Cell Receptor Excision Circles (TREC) levels. Ineligible for matched family allogeneic bone marrow (BM) transplantation, defined as the absence of a medically eligible HLA-identical sibling or family donor, with normal immune function, who could serve as an allogeneic bone marrow donor. Females of child-bearing age will be required to provide a negative pregnancy test 30 days prior to Visit 2. Subjects and their parents/legal guardians must be willing and able to comply with study restrictions and to remain at the clinic for the required duration during the study period and willing to return to the clinic for the follow up evaluation as specified in the protocol. Exclusion Criteria: Subjects will not be eligible for the study if any of the following criteria is fulfilled: Ineligible for autologous HSCT as per clinical site criteria Other conditions which in the opinion of the Principal Investigator and/or Co Investigators, contraindicate the mobilization of peripheral blood or the leukapheresis process, the administration of busulfan and the infusion of transduced cells, or which indicate an inability of the subject or subject's parent/legal guardian to comply with the protocol Hematologic abnormality, defined as: Anemia (Hb <8.0 g/dl). Neutropenia (ANC <500/mm3). Note: ANC <500 with absence of myelodysplastic syndrome on bone marrow aspirate and biopsy and normal marrow cytogenetics are acceptable for eligibility. Thrombocytopenia (platelet count <50,000/mm3, at any age). Prothrombin time or international normalized ratio (INR) and partial thromboplastin time (PTT) >2 x upper limit of normal (ULN) (subjects with a correctable deficiency controlled on medication will not be excluded). Cytogenetic abnormalities on peripheral blood or bone marrow or amniotic fluid (if available). Prior allogeneic HSCT with cytoreductive conditioning. Pulmonary abnormality, defined as: Resting O2 saturation by pulse oximetry <90% on room air. Chest X-ray indicating active or progressive pulmonary disease. Note: Chest X ray indicating residual signs of treated pneumonitis is acceptable for eligibility. Cardiac abnormality, defined as: Abnormal ECG indicating cardiac pathology. Uncorrected congenital cardiac malformation with clinical symptoms. Active cardiac disease, including clinical evidence of congestive heart failure, cyanosis, hypotension. Poor cardiac function as evidenced by left ventricular ejection fraction <40% on echocardiogram. Neurologic abnormality, defined as: Significant neurologic abnormality revealed by examination. Uncontrolled seizure disorder. Renal abnormality, defined as: Renal insufficiency: serum creatinine ≥1.2 mg/dl (106 µmol/L), or ≥3+ proteinuria. Abnormal serum sodium, potassium, calcium, magnesium or phosphate levels at >2 x ULN. Hepatic/gastrointestinal abnormality, defined as: Serum transaminases >5 x ULN. Serum bilirubin >2 x ULN. Serum glucose >1.5 x ULN. Oncologic disease, defined as: Evidence of active malignant disease other than dermatofibrosarcoma protuberans (DFSP). Evidence of DFSP expected to require anti-neoplastic therapy within the 5 years following the infusion of genetically corrected cells (if anti-neoplastic therapy has been completed, a subject with a history of DFSP can be included). Evidence of DFSP expected to be life limiting within the 5 years following the infusion of genetically corrected cells. Known sensitivity to Busulfan. Confirmation of an infectious disease by deoxyribonucleic acid (DNA) polymerase chain reaction (PCR) positive at time of assessment for the following: HIV-1, Hepatitis B, Parvovirus B19. The subject is pregnant or has a major congenital anomaly. Is likely to require treatment during the study with drugs that are not permitted by the study protocol. The subject has previously received another form of gene therapy.
Central Contact Person:
First Name & Middle Initial & Last Name or Official Title & Degree
Satiro De Oliveira, MD
Phone
1-310-825-6708
Email
sdeoliveira@mednet.ucla.edu
First Name & Middle Initial & Last Name or Official Title & Degree
Augustine Fernandes, PhD
Phone
1-310-267-4948
Email
afernandes@mednet.ucla.edu
Overall Study Officials:
First Name & Middle Initial & Last Name & Degree
Satiro De Oliveira, MD
Organizational Affiliation
Assistant Professor
Official's Role
Principal Investigator
Facility Information:
Facility Name
University of California, Los Angeles (UCLA)
City
Los Angeles
State/Province
California
ZIP/Postal Code
90095
Country
United States
Individual Site Status
Recruiting
Facility Contact:
First Name & Middle Initial & Last Name & Degree
Satiro De Oliveira, MD
Phone
310-825-6708
Email
sdeoliveira@mednet.ucla.edu
First Name & Middle Initial & Last Name & Degree
Augustine Fernandes, PhD
Phone
310-267-4948
Email
afernandes@mednet.ucla.edu

12. IPD Sharing Statement

Plan to Share IPD
No
Citations:
PubMed Identifier
24256635
Citation
Carbonaro DA, Zhang L, Jin X, Montiel-Equihua C, Geiger S, Carmo M, Cooper A, Fairbanks L, Kaufman ML, Sebire NJ, Hollis RP, Blundell MP, Senadheera S, Fu PY, Sahaghian A, Chan RY, Wang X, Cornetta K, Thrasher AJ, Kohn DB, Gaspar HB. Preclinical demonstration of lentiviral vector-mediated correction of immunological and metabolic abnormalities in models of adenosine deaminase deficiency. Mol Ther. 2014 Mar;22(3):607-622. doi: 10.1038/mt.2013.265. Epub 2013 Nov 20.
Results Reference
background
PubMed Identifier
33974366
Citation
Kohn DB, Booth C, Shaw KL, Xu-Bayford J, Garabedian E, Trevisan V, Carbonaro-Sarracino DA, Soni K, Terrazas D, Snell K, Ikeda A, Leon-Rico D, Moore TB, Buckland KF, Shah AJ, Gilmour KC, De Oliveira S, Rivat C, Crooks GM, Izotova N, Tse J, Adams S, Shupien S, Ricketts H, Davila A, Uzowuru C, Icreverzi A, Barman P, Campo Fernandez B, Hollis RP, Coronel M, Yu A, Chun KM, Casas CE, Zhang R, Arduini S, Lynn F, Kudari M, Spezzi A, Zahn M, Heimke R, Labik I, Parrott R, Buckley RH, Reeves L, Cornetta K, Sokolic R, Hershfield M, Schmidt M, Candotti F, Malech HL, Thrasher AJ, Gaspar HB. Autologous Ex Vivo Lentiviral Gene Therapy for Adenosine Deaminase Deficiency. N Engl J Med. 2021 May 27;384(21):2002-2013. doi: 10.1056/NEJMoa2027675. Epub 2021 May 11.
Results Reference
result

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Autologous Mobilized Peripheral Blood CD34+ Hematopoietic Stem and Progenitor Cells (HSPC) Transduced With the Elongation Factor Alpha Short Promoter (EFS) - Adenosine Deaminase (ADA) Gene (EFS-ADA) Lentiviral Vector for Adenosine Deaminase Severe Combined Immune Deficiency (ADA SCID)

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