Source: https://pubs.rsc.org/en/content/articlehtml/2018/nr/c8nr07424k?page=search
Timestamp: 2019-04-23 10:11:41+00:00

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Adsorption of blood proteins to the surface of nanocarriers is known to be the critical factor influencing cellular interactions and eventually determining the successful application of nanocarriers as drug carriers in vivo. There is an increasing number of reports summarizing large data sets of all identified corona proteins. However, to date our knowledge about the multiple mechanisms mediating interactions between proteins and nanocarriers is still limited. In this study, we investigate the influence of protein structure on the adsorption process and focus on the effect of heat inactivation of serum and plasma, which is a common cell culture procedure used to inactivate the complement system. As in general routine lab procedure, heat inactivation was performed at 56 °C for 30 min in order to denature heat labile proteins. When nanocarriers were exposed to native versus heat inactivated serum, we saw that the cellular uptake by macrophages was significantly affected. These results were then correlated with an altered corona composition that depended on the treatment of the protein source. In summary, we were able to prove that the protein structure is one of the key parameters determining protein corona formation.
In cell culture fetal bovine or human serum are commonly used for cell maintenance and in vitro experiments.23 Mirshafiee et al.24 and Schöttler et al.25 have already reported that protein sources such as fetal calf serum, human serum, human heparin plasma or human citrate plasma can significantly influence cellular uptake of nanocarriers and their protein adsorption patterns. Besides using the different possible cell culture supplements, it is a common procedure to inactivate the respective protein source prior to use by applying heat.26,27 During this procedure, serum is typically heated up to 56 °C for 30 min. This procedure, is aimed at inactivating heat labile proteins (e.g. complement proteins), which can interfere in immunological assays.28 Complement proteins have been identified as components of the biomolecule corona effective in a great variety of different nanocarrier formulations and they are also known to mediate interactions with immune cells.29,30 First studies regarding the influence of temperature on the formation of the protein corona were conducted by Lesniak et al.31 and Mahmoudi et al.32 In general, they found that the temperature is a crucial parameter, which affects both the protein corona composition and coverage density.
However, up to now there is still a limited knowledge about the principal mechanism, which are involved in nanoparticle–protein interaction. Next to this, the majority of literature reports do not specify whether native or heat inactivated serum was used in the experimental setup.33 In order to bridge this gap, our study specifically focuses on the effect of heat inactivation on cellular uptake and corona formation of different nanocarriers. In this study, we have been able to shed light on the role of protein structure, which critically influences the protein adsorption process. This basic knowledge is needed to unravel the process of corona formation, to streamline in vitro studies of nanocarriers, and to transfer the knowledge gained from the in vitro studies to further in vivo experiments.
Phagocytic cells such as macrophages (Fig. 1) play an important role in the immune system as they engulf foreign material (e.g. nanocarriers).34 In this study, we chose non-covalently PEGylated polystyrene nanocarriers (named as PS-PEGNC, Table S1†) as a model system to investigate the cellular interactions with a macrophage cell line (RAW264.7), as well as to study the protein adsorption behavior with regard to the heat treatment of the protein source.
Fig. 1 Heat inactivation of human serum or plasma detrimentally affects cellular uptake and protein corona formation. (A) The macrophage cell line RAW 264.7 was incubated with nanocarriers (75 μg mL−1) for 2 h, 37 °C in a protein free cell culture medium. Non-covalently functionalized PEGylated polystyrene nanocarriers (PS-PEGNC) were incubated with native or heat inactivated (56 °C, 30 min) human serum/plasma before cellular uptake experiments. The median fluorescence intensity (MFI) is shown from three biological replicates (n = 3). Values are expressed as mean ± SD. The protein corona composition was visualized by SDS PAGE (B) and quantitatively analyzed by label-free liquid chromatography-mass spectrometry (LC-MS). (C) The most abundant proteins (TOP 25) are summarized in the heat map highlighting the major protein variations. The clusterin band (marked with a red star) appears under reducing conditions at a molecular weight of 38 kDa. For statistical analysis, a one-way ANOVA using a Tukey-post hoc test was performed. *p < 0.05, **p < 0.01, ***p < 0.001.
Nanocarriers were incubated with native or heat inactivated serum and plasma (56 °C, 30 min) prior to cellular uptake studies. As a reference, cellular interaction of nanocarriers with macrophages in a protein-free medium were investigated (‘untreated’). The results corresponded with previous findings: in the presence of native serum or plasma the cellular uptake decreased strongly compared to untreated nanocarriers (Fig. 1A). This points to stealth properties induced by corona proteins.35 However, when nanocarriers were pre-coated with heat inactivated serum or plasma; we observed a significant increase in cellular uptake (***p < 0.001).
In strong contrast to this, we detected only minor amounts of clusterin in the corona (∼3%) after incubation with heat inactivated serum or plasma. Interestingly, the amounts of ApoAI remained high (Fig. 1C). In addition, the corona after incubation with heat inactivated serum and plasma was enriched with immunoglobulins (∼15%) and acute phase proteins (∼12%). Minor amounts of these proteins were identified after incubation with the native protein source (Fig. S3†).
However, there was no significant difference in the absolute amount of proteins that adsorbed to the nanocarriers after incubation with native or heat inactivated serum (Table S2†). This indicates that it is actually the protein structure (altered due to heat inactivation) that controls the distinct protein corona pattern and leads to the mediation of cellular interaction. Therefore, the increased cellular uptake after incubation with heat inactivated serum or plasma is a direct result of the altered protein corona composition (Fig. 1A).
By using label-free differential scanning fluorimetry (nanoDSF) we were able to study the unfolding process of proteins upon heating.47 The fluorescence intensity of tryptophan or tyrosine residues in a protein strongly depends on the surroundings of these amino acids and therefore changes through temperature-induced denaturation.48 In these experiments, the characteristic melting point of a protein TM is defined at a specific temperature, which is needed to unfold 50% of the protein. To explore the difference in protein corona composition when exposed to heat, the unfolding and refolding behavior of ApoAI and clusterin was investigated with nanoDSF (Fig. 2). Here, we found that clusterin had a significantly lower TM ∼ 46 °C (Fig. 2B) compared to ApoAI TM ∼ 58 °C (Fig. 2C). In addition, ApoAI was able to refold upon cooling in contrast to clusterin.
Fig. 2 Clusterin is a heat sensitive protein and readily unfolds. Differential scanning fluorimetry (nanoDSF) was used to monitor protein folding upon heating. (A) Schematic illustration of the unfolding process and exposure of tryptophan residues (here shown for human serum albumin PDB structure 1AO6). The melting temperature TM is defined as the point where 50% of the protein is unfolded. (B) Unfolding and refolding curves of clusterin in PBS (0.5 mg mL−1). The fluorescence intensity at 330 nm and the corresponding first derivative are shown. The melting temperature TM is determined from the minimum of the first derivative. One representative measurement is shown. The experiment was repeated three independent times yielding similar results. (C) Monitoring the unfolding and refolding of ApoAI in PBS (0.5 mg mL−1). One representative measurement is shown. The experiment was repeated three independent times yielding similar results. (D) Protein structure properties of clusterin and ApoAI as determined by nanoDSF. The melting point TM is given mean ± SD from three independent measurements (n = 3). The amount of unfolded protein was calculated based on the distance between the native and the denatured protein sample (90 °C) at the TM point. The denatured protein sample (90 °C) was defined as 100% unfolded.
For comparison, both proteins were incubated at 56 °C as well as 90 °C prior to taking measurements. This was done in order to determine the effect of the heat inactivation procedure and complete denaturation for reference purposes. During heat inactivation at a temperature of 56 °C for 30 min, we found that about 40% of clusterin had already unfolded, whereas the structure of ApoAI had not yet been affected. Heat inactivation at 90 °C denatured both proteins completely and irreversibly. The influence of the temperature on the protein structure was additionally analyzed by circular dichroism measurements and confirmed the results obtained from the nanoDSF measurements (Fig. S1 and S2†).
To investigate the structural involvement in protein–nanocarrier interactions still further, PS-PEGNC were incubated with the native single proteins – clusterin and ApoAI. Additionally, proteins were heated up to 56 °C or 90 °C prior to incubation in order to investigate whether temperature induced denaturation affects the binding efficiency to the nanocarriers and whether it influences cellular interaction (Fig. 3). The absolute amount of clusterin and ApoAI adsorbed to PS-PEGNC was quantified via a Pierce Assay. Here, we found that heat inactivation of the single proteins did not affect the total amount of adsorbed proteins (Fig. 3A). In addition to this, we carried out isothermal calorimetry measurements. Native or heat inactivated (90 °C) and therefore completely denatured clusterin was titrated to PS-PEGNC. Interestingly, we determined no significant differences in the binding affinity and all other binding parameters of heat inactivated clusterin compared to native clusterin with PS-PEGNC (Fig. 3B and ESI Table 4†).
Fig. 3 Structural alteration of the single proteins did not affect the biological properties whereas in a complex mixture the protein structure mediates the adsorption process. (A) Clusterin and ApoAI were heat inactivated (56 °C or 90 °C for 30 min) and incubated with PS-PEGnc for 1 h. Unbound protein was removed via centrifugation/washing and the amount of protein adsorbed to the nanocarrier surface was determined via Pierce Assay. The mean ± SD from three biological replicates (n = 3) is given. (B) Native or heat inactivated (90 °C) clusterin was titrated towards PS-PEGnc nanocarriers via isothermal titration calorimetry. The resulting integrated heats together with fits corresponding to an independent binding model are shown. (C) Cellular uptake of PS-PEGNC nanocarriers that were untreated and pre-treated with plasma, clusterin, or ApoAI towards RAW 264.7 cells (75 μg mL−1) was analyzed by flow cytometry. The median fluorescent intensity (MFI) of three biological replicates (n = 3) is shown. Values are expressed as mean ± SD. (D + E) Human serum was heated to 56 °C for 30 min. Native clusterin was further added to heat inactivated serum and the protein composition was analyzed via SDS PAGE (D) and LC-MS (E).
In order to investigate whether the stealth properties of clusterin and ApoAI (meaning the ability to prevent interaction with phagocytic cells) are affected by structural alterations, we subsequently analyzed the cellular uptake with macrophages of PS-PEGNC pre-incubated with native and heat inactivated ApoAI and clusterin. We found that pre-incubation with both proteins effectively reduced cellular uptake compared to uncoated nanocarriers. Significantly, there was no difference as to whether proteins were heat inactivated or native (Fig. 3C).
Nanocarrier behavior after incubation with single proteins contrasts strongly to incubation with the complex protein mixture (Fig. 1A). We were able to show that the interactions with native or heat inactivated serum and PEGylated nanocarriers differed strongly. We found that the abundance of clusterin within the heat inactivated serum mixture decreased dramatically in comparison to native serum.
To understand the structural involvement responsible for mediating the corona composition, serum was heat inactivated and native clusterin was re-added to the protein mixture. The protein pattern was visualized by SDS PAGE (Fig. 3D) and quantitatively analyzed by LC-MS (Fig. 3E). We found that native clusterin, which was re-added to heat inactivated serum, adsorbed to PS-PEGNC (clusterin band marked with a red star). This proves that in a complex protein mixture it is the protein structure that critically determines the adsorption behavior, which eventually affects the cellular outcome.
To further reveal the influence of the protein structure on corona formation, additional experiments were performed using a broad range of different nanocarrier systems. Here, we chose covalently PEGylated PS-NPs (PS-PEGC; Fig. S5†), carboxy- or amino-functionalized PS-NPs (PS-COOH and PS-NH2; Fig. S6†) as well as biodegradable hydroxyethyl starch nanocapsules (HES; Fig. 4 and Table S3†). All nanocarriers were incubated with native or heat inactivated serum and plasma. As in the case of PS-PEGNC there was a significant difference when particles were incubated with native serum/plasma in comparison to the heat inactivated protein source (Fig. 4A).
Fig. 4 Heat inactivation affects the adsorption behavior of complement proteins to HES nanocapsules. (A) The protein corona composition of HES nanocapsules was analyzed via SDS PAGE and LC-MS (B). Enrichment of complement proteins was detected after incubation with human serum. Due to heat inactivation, the adsorption of complement proteins was strongly diminished (C) cellular uptake of HES nanocapsules (75 μg mL−1, 2 h) by RAW264.7 cells after incubation with human serum or plasma. The amount of fluorescent positive cells (%) is shown for three biological replicates (n = 3). Values are expressed as mean ± SD. For statistical analysis a one-way ANOVA using a Tukey-post hoc test was performed. p < 0.05*, **p < 0.01, ***p < 0.001.
Proteomic analysis highlighted the major differences in the corona composition for HES nanocapsules incubated with the respective protein source (Fig. 4B). As shown above, the adsorption of clusterin was prevented when HES nanocapsules were incubated with heat inactivated serum or plasma. Additionally, we found that the corona of HES nanocapsules incubated with native serum nanocapsules was enriched with complement C3 (∼6.8%). After heat inactivation of the serum, the amount of complement C3 was strongly decreased (∼0.8%).
As widely reported, complement proteins are heat labile and undergo structural changes at 56 °C.28,49 This indicates that interactions with the nanocarriers are prevented due to the structural alterations of complement proteins (Fig. 4B).
In addition, we found major differences in the corona pattern for serum compared to plasma (Fig. 4B). As already reported in the literature, the protein source can influence corona formation.24,25 In the case of the HES nanocapsules investigated here, we detected a strong enrichment of complement proteins in the corona after serum incubation (∼15%). In contrast, significantly lower amounts of complement proteins were identified in the corona after plasma incubation (∼7%). This can be explained by the fact that complement proteins require calcium to maintain their native structure and function.50 Citrate, which was used as an anticoagulant for plasma generation in this study, specifically binds calcium.51 This suggests that the structure of the complement proteins in human plasma is different compared to that of human serum, which eventually affects the interactions of protein–nanocarriers.
Additionally, cellular uptake studies of HES nanocapsules coated with serum or plasma (native vs. heat inactivated) were able to link the distinct role of the corona composition and cellular interactions. Serum incubation strongly enhanced cellular uptake, which is mainly attributed to the involvement of complement proteins. Due to heat inactivation of serum or plasma the overall amount of complement proteins was decreased strongly, which resulted in decreased cellular interaction. Heat inactivation of plasma slightly increased cellular uptake compared to native plasma (*p < 0.05). This can probably be attributed to the lower amount of clusterin in the corona after heat inactivation, which is comparable to the results presented for PS-PEGNC.
In this study we were able to show that heat inactivation of serum or plasma critically affects cellular uptake and protein corona formation. We determined that the protein structure is, in fact, a key factor, which mediates the adsorption process. Clusterin and complement proteins were identified as heat labile proteins, which readily undergo temperature induced structural changes. Therefore, in a complex protein environment, the binding affinity of the denatured proteins to the nanocarriers was significantly decreased. In summary, the present study reveals the major role played by the protein structure and this process needs to be considered in order to unravel protein corona formation and to understand cellular interactions.
HES nanocapsules were obtained by the inverse mini emulsion process.55 The fluorescent dye sulforhodamine 101 (SR101) was in cooperated into the nanocapsules.
RAW264.7 were bought from DSMZ (Deutsche Sammlung für Mikroorganismen und Zellen, Braunschweig, Germany). The supplier provides an authentication testing. To ensure no cross-contamination, the original cells were expanded and frozen down in roughly 30 vials. Old cells were discarded every 2–3 month or after passage 25 and a new starting vial was used. Cells were maintained in Dulbecco's modified eagle medium (DMEM) supplemented with 10% FBS, 100 U ml−1 penicillin, 100 mg ml−1 streptomycin and 2 mM glutamine (Thermo Fisher) and passaged 2–3 times per week.
Cells (150 000 per well) were seeded out in 24-well plates overnight. The medium was changed to serum-free cell culture conditions for 2 h. Further nanoparticles (75 μg mL−1) were added to cells for 2 h, 37 °C. Cells were washed with PBS, detached with 0.25% Trypsin-EDTA (Gibco) and resuspended with PBS. Flow cytometry measurements were performed on a CyFlow ML cytometer (Partec). Data was analyzed by FCS Express V4 software (DeNovo Software).
Nanoparticles (0.05 m2) were incubated with 100 μg clusterin (Biozol) or apolipoprotein AI (EMD Millipore) for 1 h at 37 °C, centrifuged and further used in cell uptake experiments. Proteins were either directly used (‘native’) or heat inactivated (56 °C or 90 °C for 30 min) as indicated in the figure legend.
Serum and plasma (each bag contains a volume of ∼300 mL) was obtained from the Department of Transfusion Medicine Mainz from anonymous, healthy donors. To minimize the effect of donor specific protein alterations, serum and plasma from ten donors was pooled. The serum and plasma pools were stored in 15 mL aliquots at −80 °C.
Serum or plasma was heated up to 56 °C for 30 min and centrifuged afterwards for 30 min, 4 °C (20 000g).
Nanoparticles were incubated with the respective protein source and hard corona analysis was carried out as previously described.53 To detach proteins adsorbed to the nanoparticles, the pellet was re-suspended in 2% SDS (62.5 mM Tris·HCl). The sample was heated up to 95 °C for 5 min, centrifuged (20 000g, 4 °C, 1 h) and the supernatant was further used for protein analysis.
Nanoparticles (0.05 m2) were incubated with 100 μg Clusterin or ApoAI (native or heat inactivated as described above) for 1 h at 37 °C. Protein coated nanoparticles were purified via repetitive centrifugation and redispersion (1 mL PBS, 3 times) to remove unbound proteins. The adsorbed proteins were detached with 2% SDS (62.5 mM Tris·HCl) and the protein amount was quantified via Pierce Assay (Pierce 660 nm Protein Assay) according to the manufactures’ instruction (Thermo Fisher).
Hard corona proteins (7 μg in 26 μL) were mixed with 4 μL of NuPage Reducing Agent and 10 μL of NuPage LDS Sample Buffer NuPage. The mixture was heated up (70 °C, 10 min) and applied to a 10% Bis–Tris–Protein Gel. NuPAGE MES SDS Running Buffer was used as buffer, See Blue Plus2 Pre-Stained as molecular marker and the gel was run for 1 h at 120 V. Bands were stained with SimplyBlue SafeStain overnight and destained with distilled water for 2 h (all products Thermo Fisher Scientific).
Proteins (Clusterin and ApoAI, 0.5 mg mL−1 in PBS) were loaded into nanoDSF High Sensitivity capillaries (NanoTemper Technologies) and applied into a Prometheus NT·48 instrument. A linear thermal ramp program starting 20 °C to 95 °C (1 °C min−1) was set and the tryptophan fluorescence was measured at 330 and 350 nm. Thermal unfolding curves of the single wavelength at 330 nm and the first derivative of the fluorescence ratio (330 nm) are plotted against the temperature. The melting temperature TM is determined from the minimum of the first derivative.
Measurements were performed with a NanoITC Low Volume from TA Instruments (Eschborn) and experiments were conducted as previously described.42,60 Native or heat-treated Custerin or ApoAI was titrated towards the nanoparticle dispersion. Data was analyzed using the software NanoAnalyze.
The authors wish to thank Katja Klein for the synthesis and characterization of the nanoparticles. The authors gratefully acknowledge the financial support from the Deutsche Forschungsgemeinschaft (DFG Sonderforschungsbereich SFB 1066). Open Access funding is provided by the Max Planck Society.
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‡ These authors contributed equally.

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