Technetium-99m- or Cy7-Labeled Rituximab as an Imaging Agent for Non-Hodgkin Lymphoma

Camacho, Ximena; Machado, Camila Longo; Garcia, María Fernanda; Gambini, Juan; Banchero, A; Fernández, Marcelo; Oddone, Natalia; Zanatta, Daniela B; Rosal, Carolina; Buchpiguel, Carlos Alberto; Chammas, Roger; Riva, Eloísa; Cabral, Pablo

doi:10.1159/000452419

Cited by 17 publications

(10 citation statements)

References 36 publications

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“…27 Camacho et al also made similar observations of slow pharmacokinetics and hepatic clearance with specific NHL imaging agent 99m Tc-Hynic-rituximab. 28,29 Hence, for radioimmunodiagnosis, use of short-lived 68 Ga-labeled fragmented MAbs may be considered due to their faster pharmacokinetics, rapid clearance from body, high tumor/blood ratios, favorable imaging kinetics, better tumor penetration, lower immunogenicity, and low nonspecific binding largely owing to their small size and absence of Fc region, as compared with the intact mAbs. [30][31][32] Fragmented MAbs also allow serial imaging within a day because of shorter plasma life than intact antibody.…”

Section: Discussionmentioning

confidence: 99%

Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Suman

Kameswaran

Pandey

et al. 2019

Labelled Comp Radiopharmac

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Rituximab is used for the treatment of non‐Hodgkin lymphoma (NHL). This study focuses on development of 68Ga‐labeled rituximab fragments, (68Ga‐NOTA‐F (ab′)‐rituximab and 68Ga‐NOTA‐F (ab′)2‐rituximab, as PET‐imaging agents for NHL. Rituximab was digested with immobilized pepsin and papain to yield F (ab′)2 and Fab fragments respectively that were characterized by size exclusion HPLC (SE‐HPLC) and SDS‐PAGE. They were conjugated with p‐SCN‐Bn‐NOTA, labeled with 68Ga and characterized by SE‐HPLC. Intact rituximab was labeled with gallium‐68 for comparison. Specificity of 68Ga‐labeled immunoconjugates was ascertained by immunoreactivity and cell binding studies in Raji cells, while biodistribution studies were performed in normal Swiss mice. Gradient SDS‐PAGE under nonreducing condition showed molecular weights of F (ab′)2‐rituximab and F (ab′)‐rituximab as approximately 100 and 40 Kd, respectively. Radiochemical purity (RCP) of 68Ga‐NOTA‐F (ab′)2‐rituximab and 68Ga‐NOTA‐F (ab′)‐rituximab were 98.2 ± 0.5% and 98.8 ± 0.2% respectively with retention times of 17.1 ± 0.1 min and 19.3 ± 0.1 min in SE‐HPLC. 68Ga‐labeled rituximab fragments were stable in saline and serum up to 2‐hour post preparation and exhibited specificity to CD20 antigen. Immunoreactivity of 68Ga‐labeled immunoconjugates was greater than 80%. Clearance of the fragmented radioimmunoconjugates was predominantly through renal route. Preliminary results from this study demonstrate the potential of 68Ga‐ NOTA‐F (ab′)2‐rituximab and 68Ga‐NOTA‐F (ab′)‐rituximab as PET imaging agents for NHL.

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Section: Discussionmentioning

confidence: 99%

Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Suman

Kameswaran

Pandey

et al. 2019

Labelled Comp Radiopharmac

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“…A novel fluorescent molecule probe was first synthesized through the covalent coupling of anti-GD2 and fluorophore CyDye mono-reactive NHS esters (Cy7) ( 20 ). In the present study, according to the specific binding of antigen and antibody, synthetic anti-GD2-Cy7 wasincubated with hUC-MSCs in a standard culture medium ( 21 ). The labeled hUC-MSCs were transplanted into a lipopolysaccharide (LPS)-induced ALI mouse model to preliminarilyinvestigate the distribution processes of hUC-MSCs in treating ALI, which provides a theoretical basis for the establishment of an hUC-MSC treatment strategy for ALI in clinical work.…”

Section: Introductionmentioning

confidence: 99%

Tracking of transplanted human umbilical cord-derived mesenchymal stem cells labeled with fluorescent probe in a mouse model of acute lung injury

Geng-long

et al. 2018

Int J Mol Med

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The aim of the present study was topreliminarily visualize the distribution of humanumbilical cord-derived-mesenchymal stem cells (hUC-MSCs) in treating acute lung injury (ALI) using a targeted fluorescent technique. Anovel fluorescent molecule probe was first synthesized via the specific binding of antigen and antibody in vitro to label the hUC-MSCs. Two groups of mice, comprising a normal saline (NS)+MSC group and lipopolysaccharide (LPS)+MSC group, were subjected to optical imaging. At 4 h following ALI mouse model construction, the labeled hUC-MSCs were transplanted into the mice in the NS+MSC group and LPS+MSC group by tail vein injection. The mice were sacrificed 30 min, 1 day, 3 days and 7 days following injection of the labeled hUC-MSCs, and the lungs, heart, spleen, kidneys and liver were removed. The excised lungs, heart, spleen, kidneys and liver were then detected on asmall animal fluorescent imager. The fluorescent results showed that the signal intensity in the lungs of the LPS+MSC group was significantly higher, compared with that of the NS+MSC group at 30 min (3.53±0.06×10−4, vs. 1.95±0.05×10−4 scaled counts/sec), 1 day (36.20±0.77×10−4, vs. 23.45±0.43×10−4 scaled counts/sec), 3 days (11.83±0.26×10−4, vs. 5.39±0.10×10−4 scaled counts/sec), and 7 days (3.14±0.04×10−4, vs. 0.00±0.00×10−4 scaled counts/sec; all P<0.05). The fluorescence intensity in the liver of the LPS+MSC group, vs. NS+MSC group was measured at 30 min (0.00±0.00×10−4, vs. 0.00±0.00×10−4 scaled counts/sec); 1 day (5.53±0.08×10−4, vs. 5.44±0.16×10−4 scaled counts/sec); 3 days (0.00±0.00×10−4, vs. 8.67±0.05×10−4 scaled counts/sec); 7 days (0.00±0.00×10−4, vs. 0.00±0.00×10−4 scaled counts/sec). The signal intensity of the heart, spleen and kidneys was minimal. In conclusion, the novel targeted fluorescence molecular probe was suitable for tracking the distribution processes of hUC-MSCs in treating ALI.

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“…Hence, the absorbed dose to the tumor delivered by radionuclides with short half-lives, such as 111 In and 90 Y, is overestimated compared to those with longer half-live. We note, however, that SPECT acquisitions of mice and patients showed early uptake of rituximab in NHL [76][77] (a few hours after administration while the physical half-lives of 111 In and 90 Y are~2 days). Regarding the elimination of the rituximab in NHL, no data were found in the literature.…”

Section: Discussionmentioning

confidence: 99%

Monte Carlo dosimetry of a realistic multicellular model of follicular lymphoma in a context of radioimmunotherapy

et al. 2020

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Small-scale dosimetry studies generally consider an artificial environment where the tumors are spherical and the radionuclides are homogeneously biodistributed. However, tumor shapes are irregular and radiopharmaceutical biodistributions are heterogeneous, impacting the energy deposition in targeted radionuclide therapy. To bring realism, we developed a dosimetric methodology based on a three-dimensional in vitro model of follicular lymphoma incubated with rituximab, an anti-CD20 monoclonal antibody used in the treatment of non-Hodgkin lymphomas, which might be combined with a radionuclide. The effects of the realistic geometry and biodistribution on the absorbed dose were highlighted by comparison with literature data. Additionally, to illustrate the possibilities of this methodology, the effect of different radionuclides on the absorbed dose distribution delivered to the in vitro tumor were compared. Methods: The starting point was a model named multicellular aggregates of lymphoma cells (MALC). Three MALCs of different dimensions and their rituximab biodistribution were considered. Geometry, antibody location and concentration were extracted from selective plane illumination microscopy. Assuming antibody radiolabeling with Auger electron (125 I and 111 In) and β − particle emitters (177 Lu, 131 I and 90 Y), we simulated energy deposition in MALCs using two Monte Carlo codes: Geant4-DNA with "CPA100" physics models for Auger electron emitters and Geant4 with "Livermore" physics models for β − particle emitters. Results: MALCs had ellipsoid-like shapes with major radii, r, of~0.25,~0.5 and~1.3 mm. Rituximab was concentrated in the periphery of the MALCs. The absorbed doses delivered by 177 Lu, 131 I and 90 Y in MALCs were compared with literature data for spheres with two types of homogeneous biodistributions (on the surface or throughout the volume). Compared to the MALCs, the mean absorbed doses delivered in spheres with surface biodistributions were between 18% and 38% lower, while with volume biodistribution they were between 15% and 29% higher. Regarding the radionuclides comparison, the relationship between MALC dimensions, rituximab biodistribution and

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Technetium-99m- or Cy7-Labeled Rituximab as an Imaging Agent for Non-Hodgkin Lymphoma

Cited by 17 publications

References 36 publications

Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Tracking of transplanted human umbilical cord-derived mesenchymal stem cells labeled with fluorescent probe in a mouse model of acute lung injury

Monte Carlo dosimetry of a realistic multicellular model of follicular lymphoma in a context of radioimmunotherapy

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Technetium-99m- or Cy7-Labeled Rituximab as an Imaging Agent for Non-Hodgkin Lymphoma

Cited by 17 publications

References 36 publications

Preparation and preliminary bioevaluation studies of 68Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Preparation and preliminary bioevaluation studies of 68Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Tracking of transplanted human umbilical cord-derived mesenchymal stem cells labeled with fluorescent probe in a mouse model of acute lung injury

Monte Carlo dosimetry of a realistic multicellular model of follicular lymphoma in a context of radioimmunotherapy

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Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma

Preparation and preliminary bioevaluation studies of ⁶⁸Ga‐NOTA‐rituximab fragments as radioimmunoscintigraphic agents for non‐Hodgkin lymphoma