Evaluation of Targeted Nanoparticle Tumor Accumulation

Example 2

Mice were injected via subcutaneous injection with lymphoma cells and tumors allowed to form. Mice received intravenous (IV) injection of equal amounts of alexaflor 750-labeled ABRAXANE (ABX), ABRAXANE coated with non-specific antibodies (AB IgG), or AR160.

Twenty-four hours after IV injection, tumor accumulation of the respective treatments was determined based on a fluorescence threshold. Background was determined based on a region of the mouse without a tumor. FIG. 1 is a graphical representation of background and tumor fluorescence. Table 8 indicates the numerical values for each, including tumor-associated fluorescence (average radiant efficiency from the tumor minus background). Addition of rituximab to the ABRAXANE nanoparticle (AR160) results in a nearly 100% increase in tumor uptake of ABRAXANE.

TABLE 8

Average Radiant Efficiency and Adjusted Tumor-Associated Fluorescence

Tumor-

associated

BackgroundTumorFluorescence

ABX1.5412.090.549

AB IgG1.40051.990.5895

AR1601.5452.6371.092

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US11878061B2. Methods for improving the therapeutic index for a chemotherapeutic drug (2024-01-23). Mayo Foundation for Medical Education and Research [US]. Inventors: Svetomir N. Markovic [US], Wendy K. Nevala [US].

Patent 2024

Ab igg Abraxane Antibodies Cells Fluorescence Lymphoma Mouse Rituximab Subcutaneous injection Tumor

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Variable analysis

independent variables

Injections received by the mice
Type of ABRAXANE-based treatment

dependent variables

Tumor accumulation of the respective treatments
Tumor-associated fluorescence (average radiant efficiency from the tumor minus background)

control variables

Time between IV injection and measurement of tumor accumulation (24 hours)
Background fluorescence (determined based on a region of the mouse without a tumor)

controls

Positive control: ABRAXANE coated with non-specific antibodies (AB IgG)
Experimental treatment: ABRAXANE coated with rituximab (AR160)

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