^99mTc-Labeled Antimicrobial Peptides for Detection of Bacterial and Candida albicans Infections

Proteins, Peptides, and Ciprofloxacin

The three ubiquicidin (UBI) peptides described in this study (UBI 29–41, UBI 18–35, and UBI 31–38) were chosen because of their preferential in vitro and in vivo binding to microorganisms over host cells (5). This characteristic was also the rationale for the selection of the three lactoferrin (hLF) peptides (hLF 1–11, hLF 21–31, and hLF 4–11). The peptide hLF 4–11 was chosen as a negative control agent (5). The defensins were chosen as positive control agents for infection detection (5) and were purified from human neutrophils (12). The amino acid sequences of the various peptides are given in Table 1. Human polyclonal IgG was obtained from the Central Laboratory of the Red Cross Blood Transfusion Service (Amsterdam, The Netherlands) and served as a positive control agent for infection and inflammation (13). Stocks of the peptides were stored in 0.01% (vol/vol) acetic acid (pH 4; −20°C). Ciprofloxacin was included in this study because of its suggested specificity for bacteria (3) and was obtained from Bayer AG (Leverkusen, Germany).

Labeling Procedure and Quality Control

Antimicrobial peptides and IgG were labeled with ^99mTc as described in an earlier article (5), and ciprofloxacin was labeled with ^99mTc as described elsewhere (3). The percentage free ^99mTc activity in the labeling solutions was determined by instant thin-layer chromatography (ITLC) using saline or methyl ethyl ketone as the eluent and by high-performance liquid chromatography as described earlier (5). Because free ^99mTc activity in the solutions containing radiolabeled antimicrobial peptides and IgG (referred to as ^99mTc-labeled peptides hereafter) did not exceed 5%, no further purification was performed. Before the application of ^99mTc-labeled ciprofloxacin in the experiments, this preparation was subjected to ion-exchange Sephadex-DEAE A-25 chromatography columns (Sigma Chemical Co., St. Louis, MO) to remove free ^99mTc activity, which ranged from 20% to 40% of the total activity of the mixture. The percentage free ^99mTc activity in the labeling solutions was determined by ITLC using saline or methyl ethyl ketone as the eluent. Finally, all solutions containing ^99mTc labeling agents were diluted in phosphate-buffered saline to a concentration of 10 nmol/mL peptide or ciprofloxacin.

Microorganisms

Staphylococcus aureus 25923 and Klebsiella pneumoniae 43816 were obtained from the American Type Culture Collection (Rockville, MD), and the fluconazole-resistant Candida albicans Y01–19 was a gift from Pfizer Inc. (New York, NY). The multidrug-resistant S. aureus type 2141 (MRSA) was a clinical isolate. Overnight cultures of bacteria were prepared in brain–heart infusion broth (Oxoid, Basingstoke, U.K.) in a shaking water bath at 37°C. Overnight cultures of C. albicans were prepared in sabouraud broth (Oxoid), and they were subcultured for 2.5 h on a rotary wheel at 37°C. Virulent bacteria and C. albicans were maintained in mice. Briefly, about 1 × 10⁷ colony-forming units (CFUs) of the microorganisms were injected into the tail vein of each mouse, and 24 h thereafter the mice were killed. The spleen of each mouse was removed aseptically and homogenized, and appropriate dilutions of the homogenate were plated onto diagnostic sensitivity test agar (Oxoid), trypsone soy agar (Oxoid), or sabouraud agar (Oxoid). A single CFU was transferred into 25 mL of the appropriate broth and incubated for 24 h at 37°C. Aliquots of these suspensions containing about 5 × 10⁸ virulent microorganisms per milliliter of broth were stored at −20°C. Additionally, stocks of heat-killed bacteria or C. albicans, boiled for 2 h at 100°C, were prepared and stored at −20°C.

Animals

Specific-pathogen–free male Swiss mice (weight range, 20–25 g) and male New Zealand White rabbits (weight range, 2.5–4 kg) were used in this study. The animals were housed in the animal housing facilities of the Leiden University Medical Center for at least 1 wk before the onset of the experiments. Food and water were given ad libitum. All animal studies were performed in compliance with the local Experimental Animal Ethical Committee and the Dutch laws related to the conduct of animal experiments.

Bacterial and C albicans Infections in Mice and Rabbits

Mice were anesthetized with a single intraperitoneal injection of 0.1 mL saline containing 1 mg fluanisone and 0.03 mg fentanyl citrate (Hypnorm; Janssen Pharmaceutics, Tilburg, The Netherlands). Next, approximately 1 × 10⁷ CFUs of bacteria (S. aureus, MRSA, and K. pneumoniae) or C. albicans in 0.1 mL saline were injected into the right thigh muscle of each mouse. After 24 h, the mice were killed. The infected thigh muscles were dissected and homogenized, and the number of bacteria or C. albicans was determined microbiologically. The number of K. pneumoniae (2 × 10⁶ CFUs/g tissue) after 4 h of infection was significantly less (P < 0.05) than the number of S. aureus (2 × 10⁷ CFUs/g tissue), MRSA (8 × 10⁸ CFUs/g tissue), and C. albicans (5 × 10⁷ CFUs/g tissue). In additional studies, mice were made leukocytopenic by injecting 0.2 mL cyclophosphamide (200 mg/kg) intraperitoneally 3 d before induction of infections with 2 × 10⁵ CFUs of bacteria (S. aureus, MRSA, and K. pneumoniae). After 24 h, the number of microorganisms in the thigh muscles was comparable with the number in immunocompetent mice (0.2–8 × 10⁸ CFUs/g tissue). Blood counts were performed on randomly selected mice to confirm leukocytopenia.

Selected peptides were also applied in rabbits with an experimental infection. In short, the rabbits were injected with 0.4 mL saline containing 1 × 10⁷ CFUs of bacteria (S. aureus, MRSA, and K. pneumoniae) into the right thigh muscle or into the right front leg muscle. The rabbits were anaesthetized 18 h thereafter by a single injection of 0.4 mL saline containing 4 mg fluanisone and 0.13 mg fentanyl citrate into the left thigh muscle.

Inflammatory Processes in Mice and Rabbits

The accumulation of radiolabeled tracers was also studied in animals with a sterile inflammatory process to select compounds with a low accumulation in inflamed tissues that may discriminate between infection and sterile inflammation. Mice and rabbits were anaesthetized as described previously. Sterile inflammation was induced 18 h before administration of the tracer by an intramuscular injection of 0.1 mL saline containing either 1 mg lipopolysaccharide (LPS) or approximately 2 × 10⁸ heat-killed bacteria or C. albicans. Eighteen hours after injection with both stimuli, we observed a significant increase (>60%; P < 0.001) in the weight of the injected thigh muscle compared with the contralateral thigh muscle.

Scintigraphy

Animals were anaesthetized 18 h after infection as described previously, and 0.1 mL labeling solution containing 1 nmol peptide or anti-infective was injected into a tail vein. The accumulation of the radiolabeled peptides, ciprofloxacin, and IgG in the bacterial or C. albicans infected muscles in mice and rabbits was assessed by planar scintigraphy. Before scintigraphy, a subcutaneous injection of 0.05 mg diazepam (Valium; Hoffmann-Roche, Mijdrecht, The Netherlands) in 0.1 mL saline was administered to the mice to induce muscle relaxation. Next, the animals were placed in a supine position on a collimator of a planar gamma camera with both hind legs spread out and fixed with surgical tape. Continuous anterior whole-body acquisitions of the animals every 60 s during the first 2 h after injection and a single static acquisition at 4 h after injection of the tracer were made. On the scintigrams, anatomically adjusted regions of interest were drawn over the entire infected or inflamed muscle (target) and the contralateral muscle (nontarget). The accumulation of ^99mTc-labeled tracers at sites of infection or inflammation is expressed as the ratio of the counts in the target muscle to the counts in the nontarget muscle (T/NT). Scintigraphic data were interpreted by two observers, and the results were always similar to the data obtained after obduction, as described later. When scintigraphic data from the two sessions differed, we used T/NT obtained after obduction. For comparison of the accumulation of the various ^99mTc-labeled compounds, we calculated the mean ± SEM of T/NT at 30, 60, and 120 min after injection of the tracers into the mice with infected or inflamed thigh muscles. The animals were killed 4 h after tracer injection by an intraperitoneal injection of 0.5 mL (mice) or 5 mL (rabbits) sodium barbiturate (60 mg/mL saline, Nembutal; Sanofi BV, Division Algin, Maassluis, The Netherlands). Next, the entire infected and noninfected thigh muscles were removed, weighed, and counted for radioactivity, and T/NT was calculated.

Statistical Analysis

Differences in the data were evaluated with the Student t test. Results for the probability value using the 2-tailed test are reported, and all results are given as mean ± SEM.

Detection of Bacterial Infections in Mice

The sites of bacterial infections could be visualized within 1 h after injection of the ^99mTc-labeled peptides. Typical scintigrams for UBI 29–41 and hLF 1–11 in S. aureus infected mice are depicted in Figure 1. The accumulation of ^99mTc-labeled UBI 29–41 in the thigh muscle of mice infected with various microorganisms is shown in Figure 2. Within the period of analysis, significantly higher T/NT was observed for ^99mTc-labeled UBI peptides as well as for hLF 1–11, hLF 21–31, and the defensins in infected thigh muscles compared with T/NT measured in sterile inflammatory sites (Table 2). The accumulation of ciprofloxacin (Fig. 1) and ^99mTc-labeled hLF 4–11 in infected tissues was comparable and showed no significant difference between bacterial infections and sterile inflammatory sites. In a small group of randomly selected animals, we determined T/NT also from data obtained with entirely dissected thigh muscles. The comparison of these data revealed similar T/NT after calculations from scintigraphic data (results not shown).

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FIGURE 1.

Typical scintigrams of ^99mTc-labeled UBI 29–41 (A), hLF 1–11 (B), ciprofloxacin (C), and human polyclonal IgG (D) 1 h after injection into mice having thigh muscles infected with S. aureus.

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FIGURE 2.

Accumulation of ^99mTc-labeled antimicrobial peptide UBI 29–41 in thigh muscles of mice infected with MRSA (white bars), K. pneumoniae (square-hatched bars), or fluconazole-resistant C. albicans (black bars). Furthermore, mice were injected intramuscularly with LPS (diagonally hatched bars) or heat-killed bacteria (horizontally hatched bars) 18 h before administration of tracer. Each symbol at each time point represents mean ± SEM T/NT of at least 12 animals obtained from three independent experimental settings.

To investigate whether the accumulation of the tracers depends on the binding to infiltrating leukocytes, we determined T/NT for the various ^99mTc-labeled UBI peptides in leukocytopenic mice with an MRSA or K. pneumoniae infection. These data were compared with the respective values of accumulation in immunocompetent mice. The results revealed no significant differences in intensity and rate of accumulation of the ^99mTc-labeled peptides in the infected tissues of leukocytopenic and immunocompetent mice. This finding indicated that the accumulation of radiolabeled UBI peptides is not dependent on the interaction of these tracers with infiltrating leukocytes.

Detection of Infection with C. albicans in Mice

Immunocompetent mice were used to study the accumulation of ^99mTc-labeled peptides, ciprofloxacin, and IgG in experimental thigh muscle infections with C. albicans. On the scintigrams, the C. albicans infections in the thigh muscles of mice could be seen within 1 h after injection of ^99mTc-labeled compounds. For example, the time-dependent accumulation of various tracers in the thigh muscles of mice infected with viable C. albicans is shown in Figure 3. At 30 min after injection, all tracers visualized the infected thigh muscles, and the mean T/NT over the interval from 30 to 120 min after injection was high for all tracers tested (Table 2).

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FIGURE 3.

Accumulation of ^99mTc-labeled UBI 29–41 (white bars), UBI 18–35 (square-hatched bars), hLF 1–11 (horizontally hatched bars), ciprofloxacin (black bars), and IgG (checkered bars) in thigh muscles of mice infected 18 h earlier with fluconazole-resistant C. albicans. Each symbol at each time point represents mean ± SEM T/NT of at least six animals obtained from three independent experimental settings.

Sterile Inflammations in Mice

The accumulation of radiolabeled tracers was also studied in animals with sterile inflammatory processes to select compounds that discriminate between infection and sterile inflammation. The results for typical scintigrams of various radiolabeled tracers in mice with thigh muscles injected with heat-killed S. aureus are shown in Figure 4. Good accumulation in mice with sterile inflammatory processes (induced by injections with LPS or heat-killed microorganisms) was observed for ^99mTc-labeled ciprofloxacin and IgG (Fig. 4).

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FIGURE 4.

Typical scintigrams of ^99mTc-labeled UBI 29–41 (A), hLF 1–11 (B), ciprofloxacin (C), and human polyclonal IgG (D) 1 h after injection into mice having thigh muscles injected with heat-killed S. aureus.

Bacterial Infections in Rabbits

Because of the favorable results in mice, we assessed the accumulation of the ^99mTc-labeled peptides UBI 29–41, UBI 18–35, and UBI 22–35 in rabbits with bacterial infections of the thigh muscle or front leg muscle. Figure 5A is a scintigram of a rabbit with a K. pneumoniae infection in the thigh muscle 1 h after injection of ^99mTc-labeled UBI 29–41. Figure 5B is the same scintigram with lower contrast to depict the biodistribution of this peptide 1 h after injection. The highest T/NT in rabbits was observed 4 h after injection of ^99mTc-labeled peptides; for example, for UBI 29–41 (Fig. 6), the highest T/NT was approximately 6. Two rabbits with a K. pneumoniae infection in the front leg were injected with ^99mTc-IgG, and the infected area became visible 2 h after injection. The highest values of T/NT (4–5) of ^99mTc-IgG in infected tissues were observed 4 h after injection (data not shown).

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FIGURE 5.

(A) Typical scintigram of ^99mTc-labeled UBI 29–41 1 h after injection into rabbits with thigh muscles infected with S. aureus. (B) Biodistribution of ^99mTc-labeled UBI 29–41 1 h after injection with lower contrast.

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FIGURE 6.

Accumulation of ^99mTc-labeled UBI 29–41 in thigh muscles of rabbits injected with MRSA (white bars), K. pneumoniae (square-hatched bars), heat-killed MRSA (diagonally hatched bars), heat-killed K. pneumoniae (horizontally hatched bars), or 50 mg LPS (black bars). Each symbol at each time point represents mean ± SEM T/NT of at least three animals obtained from independent experimental settings.

Sterile Inflammations in Rabbits

As observed in mice, the ^99mTc-labeled UBI peptides did not visualize inflamed thigh muscles or front leg muscles in rabbits (Fig. 6).