Systemic targeted radiotherapy is an evolving and promising modality of cancer treatment. The goal of systemic targeted radiotherapy is to be efficacious, yet with minimal normal tissue toxicity. The key characteristic of systemic targeted radiotherapy is that a molecule (antibody, antibody fragment, or peptide) can deliver higher amounts of a radionuclide to cancer cells than to normal tissue. Unlike chemotherapy, systemic targeted radiotherapy is cancer cell specific.
The radiopharmaceutical used by Chen et al. (1) in this issue of The Journal of Nuclear Medicine is 111In-DTPA-NLS-HuM195 (DTPA is diethylenetriaminepentaacetic acid; NLS is See page 827
nuclear localizing sequence). HuM195 is a humanized IgG1 monoclonal antibody (mAb) that targets the CD33 antigen on acute myeloid leukemia cells. By itself, HuM195 is not toxic but it effectuates cell killing as a toxin carrier. HuM195 is in current clinical use as Mylotarg (Wyeth-Ayerst; HuM195 conjugated with gemtuzumab ozogamicin, a chemotherapy agent). Despite the enticing ability to target leukemia cells with Mylotarg, the complete response rate is only 26% and patients who do respond ultimately relapse (2). Another part of 111In-DTPA-NLS-HuM195 is the NLS, a peptide (CPYGPKKKRKVGG) derived from the simian virus 40 large T-antigen. This is a unique use of biology; the peptide sequence of a virus (which facilitates viral genome entry into its target cell) is now being used in a positive way, to allow entry of a radiopharmaceutical into the malignant cell nucleus. DTPA is used to chelate 111In, the therapeutic radionuclide.
131I and 90Y are commonly used therapeutic radionuclides (3). The β-particles of these radionuclides are responsible for their efficacy as well as toxicity. Despite specificity, systemic radiation therapy as usually delivered does have toxicity, with myelotoxicity being predominant. Nonhematologic toxicity is usually minimal, thereby giving hope that this form of therapy can be improved to create a truly specific, effective, yet nontoxic, therapy applicable to patients with different kinds of cancer. It is this hope that makes the publication by Chen et al. (1) encouraging.
The article by Chen et al. (1) is exciting not only because of the data that it presents but also because of its concepts. The basic strategy starts with the HuM195 anti-CD33 mAb to specifically target myeloid leukemia cells. HuM195 is rapidly internalized into targeted cells; internalization is one of the first requirements for this strategy to be successful. Many other antibodies are also rapidly internalized into the cytoplasm after cell-surface receptor binding. The innovative part of this new strategy is that NLS have been conjugated to the antibody. Thus, what is transported into the cell cytoplasm is a drug that has secondary targeting ability—namely, it targets the cancer cell nucleus and is transported through the nuclear membrane. In that way, HuM195 will be in close contact with the DNA. This provides a great opportunity for a new kind of targeted therapy. Because the antibody has been able to enter the nucleus, drugs that work by contact with DNA have an opportunity to be effective. In this case, 111In was used to kill malignant cells through direct DNA damage. This was a logical choice of radionuclides because the Auger electrons have only a nanometer-to-micrometer range that is long enough to damage DNA in the malignant cells, but not so long as to damage surrounding normal cells. In addition, the decay product of 111In is cadmium, which is stable, unlike the decay products of other potentially useful radionuclides. This is different than standard systemic targeted radiotherapy where “normal bystander” cells along with the cancer are killed by β-particles.
It is easy to see the therapeutic possibilities of cancer cell–nuclear targeting as it is developed into drugs for patients. For example, for a therapy to be curative, virtually all malignant cells must be killed. However, it is difficult to completely eliminate cancer because of the therapy's toxicity. 111In-NLS-mAb could be a way to eradicate minimal residual disease. Because it would be specific and because the accompanying toxic drug would itself not be very destructive outside of the cell nucleus, cancer-specific nuclear targeting would be able to effectively target and kill residual cancer cells. This is similar in some ways to traditional radioimmunotherapy because that also involves the use of a specific antibody carrying a radionuclide. However, with traditional radioimmunotherapy, the typical radionuclides (90Y, 131I, 67Cu) have significant toxicity in the amounts used. Relatively long-range β-emissions that can damage normal cells are a particular problem with hematologic malignancies, where the bone marrow may harbor malignant cells. The “normal bystander effect” (death of normal cells near targeted malignant cells) is a problem solved with the strategy described in the publication by Chen et al. (1). Radiation safety is also an important issue for patients receiving radioimmunotherapy. This study uses 111In, which does not have some of the radiation safety issues that are encountered with 131I-containing radiopharmaceuticals. In addition, there is little danger to the thyroid from 111In as there is with 131I. Clearance of a radionuclide is always an important consideration with radiopharmaceuticals. 131I is predominantly cleared from the body in the urine; with 90Y-containing radiolabeled antibodies, much of the radionuclide is retained in the body. If modest doses of 111In-NLS-mAb are used, differences in radiopharmaceutical clearance between patients are likely to have less impact on the development of clinical side effects. The lower toxicity with this strategy is due to the use of 111In and the fact that it is likely that the radiopharmaceutical will be retained within the nucleus of the targeted cell. In addition, because a targeting construct and NLS will be able to enter the nuclei of malignant cells, several other interesting agents could be attached to kill cells—for example, drugs that could target specific genes and chemotherapy drugs.
The accompanying publication conclusively showed that the conjugation of 4–8 NLS peptides to the 111In-DTPA-HuM195 mAb increased uptake of 111In into the nucleus, retained specificity, killed leukemia cells, and did not produce toxicity in mice. Of course, almost anything is toxic if enough is administered; that is the point of developing the sort of radiopharmaceuticals described by Chen et al. (1)—they enter the nucleus of malignant cells so high doses may not be needed. The radiation-absorbed dose of 111In is 34 times higher when it decays in the nucleus than on the cell surface (4). The Auger electrons of 111In are potent and cytotoxic when they decay in the cell nucleus (5). The uptake of radiopharmaceutical into the nucleus was increased by increasing the numbers of conjugated NLS, but the affinity of the mAb for cellular targeting was not significantly diminished by up to 12 NLS.
In conclusion, advances in therapy frequently arise one step at a time. A mAb, radionuclide, chelator, and NLS are all part of 111In-DTPA-NLS-HuM195. This may develop into an important new drug and concept that will be translated into better cancer therapy.
References
- Received for publication January 18, 2006.
- Accepted for publication January 23, 2006.