The Gd-DTPA
MRI signals depend on a wide range of parameters. The key factor of conventional MRI contrast is the interaction of the total water signal (proton density) and the magnetic properties of the tissues (2, 3). Various paramagnetic and superparamagnetic contrast agents can increase the sensitivity and specificity of MRI. Current clinical agents are predominately Gd-based contrast agents (GBCA) and are largely nonspecific, low molecular weight compounds. These agents have transient tissue retention, a wide distribution into the extracellular space, and rapid excretion from the body (3-5). There is a need to develop intravascular MRI contrast agents that have a sufficiently long intravascular half-life (t½) to allow imaging of the vasculature and aid in the detection of cancer and cardiovascular diseases (6, 7).
Current strategies to prolong the intravascular t½ include the chelation of paramagnetic ions to macromolecules and the use of superparamagnetic nanoparticles (1, 6, 7). Macromolecular contrast agents are generally large enough (>20 kDa) so that they do not readily diffuse across the healthy vascular endothelium and are not rapidly excreted. These agents are retained in the vasculature for a sufficiently prolonged period of time to allow for imaging, and they also preferentially accumulate in disease tissues with leaky vasculature, such as cancers and vascular disease. Most macromolecular GBCAs are prepared by the conjugation of Gd3+ chelates to biomedical polymers including poly(amino) acids (8, 9), polysaccharides (10, 11), dendrimers (12, 13), and proteins (14), or by the copolymerization of diethylenetriamine pentaacetic acid (DTPA) dianhydride with diamines and the complexation with Gd3+ (15, 16). However, the development of these macromolecular GBCAs has been hampered by potential Gd toxicity associated with the slow degradation of chemically modified biomedical polymers (6, 17). Smaller macromolecules (<20 kDa) are cleared more rapidly by the kidneys but their effectiveness may also be compromised. One approach to improve the safety of macromolecular GBCAs is the development of small molecules (<1.2 kDa) with a hydrophilic Gd3+ complex and a hydrophobic region for reversible noncovalent binding to serum albumin (6, 18). Lu et al. (17, 19) proposed another approach by designing biodegradable macromolecular polydisulfide GBCAs. These agents have disulfide bonds incorporated into a polymeric backbone, and these bonds can be readily reduced by the thiol-disulfide exchange reaction with endogenous or exogenous thiols, such as glutathione and cysteine. As a result, these macromolecules are broken down into smaller complexes that are readily excreted by the kidneys. The Gd-DTPA-cystamine copolymer was the first such agent synthesized by the copolymerization of cystamine and DTPA dianhydride (17). A series of polydisulfide-based macromolecular GBCAs with different structural modifications around the disulfide bonds have been synthesized and evaluated by the same research team of Lu et al. (17, 20-23). Kaneshiro et al. (1) reported the synthesis and evaluation of GCPC and two other derivatives (GCAC and GCIC) with different amide substituents at the cystine carboxylic groups. All three neutral agents were cleaved in vivo into low molecular weight Gd3+ chelates and were cleared rapidly in rats.
Both renal and extrarenal toxicities have been reported after the clinical use of GBCAs in patients with underlying kidney disease (24-26). In 2007, the