Ies, their limitations and the essential steps required for successful future development. The design, synthesis and utility of such customizable targeting probes will also be discussed in this section. Aside from light penetration, a specific limitation for deep tissue PDT is the inadequate tissue selectivity of phototoxicity. Although phototoxicity is confined to areas of irradiation, cellular discrimination of PDT within those areas is typically poor as a result of weak PS selectivity and strong tissue scattering of the excitation light. When irradiating neoplastic tissue in the vicinity of sensitive anatomical sites, such as the brain, off target phototoxicity could have drastic undesired effects, reducing the maximum tolerated PDT dose and limiting efficacy. This was exemplified by an in vivo canine brain tumor PDT study where high-dose therapy using 1800 J of 630 nm light and 2-4 mg/kg of the PS photofrin induced Nectrolide site significant neurotoxicity and brain stem damage [119]. Reducing the administered PS dose to 0.75 mg/kg eliminated these adverse effects. Thus, selectivity of phototoxicity can be achieved by confining photosensitization to diseased tissue cells by targeting the PSs, regardless of the off-target incident light, thereby increasing the maximal tolerated PDT doses. The critical parameters required for successful deep-tissue PDT are common for most bioconjugated diagnostic and therapeutic probes. These parameters revolve around the biological targeting probe’s molecular weight, immunological effects dictating itshttp://www.thno.orgTheranostics 2016, Vol. 6, Issuecirculation times, physiological clearance rates, physiological impact following PS conjugation, and the optical properties that ultimately govern their effectiveness as deep-tissue PDT agents. PS targeting can be achieved through three archetypal probe platforms as illustrated in Fig. 6, which will be discussed in this section. These platforms include probes for targeted delivery, probes for tumor-selective activation and probes that combine selective delivery and activation.PIC platform have since been developed, including multiple PS molecules stochastically conjugated to antibodies using similar covalent coupling techniques [121-127]. Both the glycosylation sites on the Fragment crystallizable (Fc) portion of full-length antibodies and the hinge region disulfides have been frequently utilized as handles for the site-specific conjugation of polymers carrying PS payloads so as to avoid PS A-836339 custom synthesis interference with the antibody’s binding capacity [128-132]. Since the seminal work by Levy et al., targeted imaging and fluorescence-guided surgical debulking assisted by an improved tumor margin delineation has attracted attention in the clinic. The clinical ambition of targeted theranostic probes modified with photosensitizing agents ultimately lies in the accurate photodiagnosis of malignant tissue followed by its selective PDT eradication. Towards this goal, fluorescent targeting probes have been clinically deployed for the surgical assistance of tumor resection. The earliest clinical use of targeted photoactive probes for the optical detection of cancer tissue in patients was reported in 1992 by Folli et al. who utilized a fluorescein conjugate of an anti-carcinoembryonic antigen antibody [115]. Although not used to intraoperatively assist surgical resection of the colonic carcinomas, in vivo selectivity of the probe was validated by ex vivo fluorescence imaging revealing hete.Ies, their limitations and the essential steps required for successful future development. The design, synthesis and utility of such customizable targeting probes will also be discussed in this section. Aside from light penetration, a specific limitation for deep tissue PDT is the inadequate tissue selectivity of phototoxicity. Although phototoxicity is confined to areas of irradiation, cellular discrimination of PDT within those areas is typically poor as a result of weak PS selectivity and strong tissue scattering of the excitation light. When irradiating neoplastic tissue in the vicinity of sensitive anatomical sites, such as the brain, off target phototoxicity could have drastic undesired effects, reducing the maximum tolerated PDT dose and limiting efficacy. This was exemplified by an in vivo canine brain tumor PDT study where high-dose therapy using 1800 J of 630 nm light and 2-4 mg/kg of the PS photofrin induced significant neurotoxicity and brain stem damage [119]. Reducing the administered PS dose to 0.75 mg/kg eliminated these adverse effects. Thus, selectivity of phototoxicity can be achieved by confining photosensitization to diseased tissue cells by targeting the PSs, regardless of the off-target incident light, thereby increasing the maximal tolerated PDT doses. The critical parameters required for successful deep-tissue PDT are common for most bioconjugated diagnostic and therapeutic probes. These parameters revolve around the biological targeting probe’s molecular weight, immunological effects dictating itshttp://www.thno.orgTheranostics 2016, Vol. 6, Issuecirculation times, physiological clearance rates, physiological impact following PS conjugation, and the optical properties that ultimately govern their effectiveness as deep-tissue PDT agents. PS targeting can be achieved through three archetypal probe platforms as illustrated in Fig. 6, which will be discussed in this section. These platforms include probes for targeted delivery, probes for tumor-selective activation and probes that combine selective delivery and activation.PIC platform have since been developed, including multiple PS molecules stochastically conjugated to antibodies using similar covalent coupling techniques [121-127]. Both the glycosylation sites on the Fragment crystallizable (Fc) portion of full-length antibodies and the hinge region disulfides have been frequently utilized as handles for the site-specific conjugation of polymers carrying PS payloads so as to avoid PS interference with the antibody’s binding capacity [128-132]. Since the seminal work by Levy et al., targeted imaging and fluorescence-guided surgical debulking assisted by an improved tumor margin delineation has attracted attention in the clinic. The clinical ambition of targeted theranostic probes modified with photosensitizing agents ultimately lies in the accurate photodiagnosis of malignant tissue followed by its selective PDT eradication. Towards this goal, fluorescent targeting probes have been clinically deployed for the surgical assistance of tumor resection. The earliest clinical use of targeted photoactive probes for the optical detection of cancer tissue in patients was reported in 1992 by Folli et al. who utilized a fluorescein conjugate of an anti-carcinoembryonic antigen antibody [115]. Although not used to intraoperatively assist surgical resection of the colonic carcinomas, in vivo selectivity of the probe was validated by ex vivo fluorescence imaging revealing hete.