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Tumor imaging and targeting potential of an Hsp70-derived 14-mer peptide

PLoS ONE (2014) 9(8)
DOI: 10.1371/journal.pone.0105344
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Abstract

Background: We have previously used a unique mouse monoclonal antibody cmHsp70.1 to demonstrate the selective presence of a membrane-bound form of Hsp70 (memHsp70) on a variety of leukemia cells and on single cell suspensions derived from solid tumors of different entities, but not on non-transformed cells or cells from corresponding 'healthy' tissue. This antibody can be used to image tumors in vivo and target them for antibody-dependent cellular cytotoxicity. Tumor-specific expression of memHsp70 therefore has the potential to be exploited for theranostic purposes. Given the advantages of peptides as imaging and targeting agents, this study assessed whether a 14-mer tumor penetrating peptide (TPP; TKDNNLLGRFELSG), the sequence of which is derived from the oligomerization domain of Hsp70 which is expressed on the cell surface of tumor cells, can also be used for targeting membrane Hsp70 positive (memHsp70+) tumor cells, in vitro. Methodology/Principal Findings: The specificity of carboxy-fluorescein (CF-) labeled TPP (TPP) to Hsp70 was proven in an Hsp70 knockout mammary tumor cell system. TPP specifically binds to different memHsp70+ mouse and human tumor cell lines and is rapidly taken up via endosomes. Two to four-fold higher levels of CF-labeled TPP were detected in MCF7 (82% memHsp70+) and MDA-MB-231 (75% memHsp70 +) cells compared to T47D cells (29% memHsp70+) that exhibit a lower Hsp70 membrane positivity. After 90 min incubation, TPP co-localized with mitochondrial membranes in memHsp70+ tumors. Although there was no evidence that any given vesicle population was specifically localized, fluorophore-labeled cmHsp70.1 antibody and TPP preferentially accumulated in the proximity of the adherent surface of cultured cells. These findings suggest a potential association between membrane Hsp70 expression and cytoskeletal elements that are involved in adherence, the establishment of intercellular synapses and/or membrane reorganization. Conclusions/Significance: This study demonstrates the specific binding and rapid internalization of TPP by tumor cells with a memHsp70+ phenotype. TPP might therefore have potential for targeting and imaging the large proportion of tumors (∼50%) that express memHsp70. © 2014 Gehrmann et al.

Figures

  • Figure 1. Tumor cell lines expressing memHsp70 are able to bind TPP at 46C. The memHsp70 status of a panel of human breast, colon, melanoma, lung, head & neck tumor cell lines was assessed using the cmHsp70.1 antibody (top row histograms). Incubation of tumor cells with carboxyfluorescein (CF)-labeled TPP at 4uC (bottom row histograms) results in a similar binding profile to that of cmHsp70.1 antibody in all tumor cell lines; grey, isotype controls, open histograms, Hsp70 specific reagents. The numbers in the histograms show the proportion of Hsp70 membranepositively stained cells. doi:10.1371/journal.pone.0105344.g001
  • Figure 3. TPP specifically binds to Hsp70, but not to other Heat shock proteins (HSPs). A peptide ELISA was performed to determine the in vitro binding capacity of peptides to different HSPs. Ninety six well plates that were coated either with Hsp70, Hsp60, Grp78, or Hsp27 were incubated with carboxyfluorescein (CF)-labeled TPP or a scrambled peptide at concentrations ranging from 100 to 25 ng/ml. Fluorescence was measured after 30 min at 27uC using a multiplate reader. Combinations of peptides and proteins are indicated as ‘‘+’’ in the lower panel. Differences in peptide binding (100 ng/ml) were evaluated using the Student’s t-test (** p,0.01; *** p,0.001) (n = 3). doi:10.1371/journal.pone.0105344.g003
  • Figure 4. Specific uptake of TPP into tumor cells at 376C. Human breast cancer cell lines expressing different levels of memHsp70 (MCF7, MDA-MB-231, T47D) were incubated with CF-labeled TPP or a scrambled peptide for 30 min at 37uC and the internalization of peptides imaged using confocal microscopy. A. TPP (green, right panel), but not the scrambled peptide (left panel) is internalized into the tumor cell lines. The appearance of the TPP (green, right panel) in well-defined, localized points suggests that the association of the peptide with intracellular vesicles is related to the memHsp70 expression status. The numbers shown as inserts indicate the percentage of memHsp70 positively stained cells. DAPI staining allows visualization of the nucleus (blue). Objective 26; scale bar 50 mm. B. Individual cells were imaged as a z-stack in order to better illustrate the intracellular localization of TPP. Images are representative three-frame composites from approximately mid-way in the stack. Immunofluorescence staining, (left panel); brightfield, (right panel). Objective 636; scale bar 10 mm. doi:10.1371/journal.pone.0105344.g004
  • Figure 5. Kinetics of TPP internalization. (Left panel) Flow cytometric analysis of memHsp70 positive human breast cancer lines MCF7, MDA-MB231, T47D reveals an accumulation of the fluorescence intensity after incubation with CF-labeled TPP at 37uC between 1 and 60 min (solid lines). At 4uC (dashed lines) mean fluorescence intensity remained low within the same time frame. Cell lines with a high percentage of Hsp70 membrane positive cells (MCF7, MDA-MB-231) exhibit a higher and more rapid uptake of TPP, whereas the cell line with low Hsp70 membrane expression (T47D) exhibits only a low uptake of TPP. (Right panel) Confocal microscopy images were analyzed to provide a total count of fluorescent spots per cell after incubation with the TPP at 37uC for 30 min. Although fluorescent spots progressively accumulated in all three cell lines, this was most apparent in the MCF7 and MDA-MB-231 cell lines that express higher levels of memHsp70 than T47D cells. doi:10.1371/journal.pone.0105344.g005
  • Figure 7. Localization of internalized TPP within cells. Confocal microscopy z-stacks were used to divide cells into quartiles using percentages of cell height from the adherent interface (0%) to the apex of the cells (100%). The number of fluorescent TPP spots in each quartile was counted in order to quantify the peptide distribution. For all time points and all cell lines investigated, TPP spots were found to be more prevalent in the quartile which included the adherent surface. This finding suggests that TPP is preferentially internalized and trafficked via this interface. The data shown are representative composite images of every z-stack frame counted in each quartile. Images were produced using a 636/1.4 oil immersion lens on an inverted Zeiss 510 confocal microscope. doi:10.1371/journal.pone.0105344.g007
  • Figure 8. Distribution of intracellular vesicles in MCF7 cells. MCF7 tumor cells grown in glass-bottomed MatTek dishes for 48 h were fixed in paraformaldehyde, permeabilized and stained with primary antibodies specific for early (Rab4, Rab5), late (Rab7, Rab9) and recycling (Rab11) endosomes or lysosomes (LAMP1), followed by an appropriate Cy3-labeled secondary antibody (red). The nucleus was counter-stained with DAPI (blue). Representative three-frame composites from across the z-stack are shown. All of the vesicular markers assessed were found to be homogenously distributed throughout the cells. Objective 636; scale bar 10 mm. doi:10.1371/journal.pone.0105344.g008
  • Figure 9. Uptake of TPP between 0 and 60 min follows an endosomal pathway. MCF7 cells take up CF-labeled TPP via an endosomal transport route in a time-dependent manner. Co-localization of TPP (green) with the endosomal marker proteins (Rab5, Rab7, LAMP1; each in red) is visible as a yellow signal. Co-localization of TPP with Rab5 can be seen within early endosomes at early time points (,30 min, arrows, upper left graph), but not at later time points (arrow heads, upper right graph). Between 30 and 60 min, TPP co-localizes with Rab7 vesicles (arrows, lower left graph). After 60 min, TPP co-localizes with LAMP1 positive lysosomes (arrows, lower right graph). Images are representative three-channel composites: brightfield, FITC, RFP. Objective 636; scale bar 10 mm. doi:10.1371/journal.pone.0105344.g009
  • Figure 10. TPP co-localizes with mitochondria after 90 min. MCF7, MDA-MB-231, and T47D cells were incubated with CF-labeled TPP (green) for 90 min, stained with the mitochondrial detection dye Mito-ID (purple) and then imaged using confocal microscopy. A proportion of internalized TPP co-localizes with mitochondria in all three tumor cell lines (Pearson’s coefficient: MCF7 r = 0.855, MDA-MB-231 r = 0.585, T47D r = 0.813). The Manders’ M1 coefficient was used to estimate the proportion of total TPP that co-localizes with mitochondria (40% in MCF7 cells, M1 = 0.407; 44% in MDA-MB-231 cells, M1 = 0.443). In contrast, 14% of TPP was co-localized to mitochondria in T47D cells (M1 = 0.141). These findings correlate with the differential Hsp70 membrane expression levels of the respective cancer cell lines. Images are representative single frames. Objective 636; scale bar 10 mm. doi:10.1371/journal.pone.0105344.g010

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Gehrmann, M., Stangl, S., Foulds, G. A., Oellinger, R., Breuninger, S., Rad, R., … Multhoff, G. (2014). Tumor imaging and targeting potential of an Hsp70-derived 14-mer peptide. PLoS ONE, 9(8). https://doi.org/10.1371/journal.pone.0105344

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