An innovative consolidation strategy for degraded paper is presented based on the reversible application of cellulose nanocrystals as sustainable fillers to reinforce mechanical properties and resistance to further degradation. The compatibility and efficacy of the proposed consolidation treatment are assessed first on pure cellulose paper, used as a model, by reliable techniques such as field emission scanning electron microscopy, atomic force microscopy, tensile tests, X-ray powder diffraction, and Fourier transform infrared spectroscopy, evidencing the influence of the surface functionalization of nanocellulose on the consolidation and protection effects. Then, the consolidation technique is applied to real aged paper samples from Breviarium romanum ad usum Fratrum Minorum S.P. ( 1738), demonstrating the promising potential of the suggested approach. Amperometric measurements, carried out with a smart electrochemical tool developed in our laboratory, demonstrate the reversibility of the proposed treatment by removal of the nanocrystalline cellulose from the paper surface with a suitable cleaning hydrogel. This completely new feature of the consolidation treatment proposed here satisfies a pivotal requisite in cultural heritage conservation because the methodological requirement for the ″reversibility″ of any conservation measure is a fundamental goal for restorers. A paper artifact, in fact, is subject to a number of natural and man-made hazards, inducing continuous degradation. With time, monitoring and consolidation actions need to be often performed to ensure conservation, and this tends to modify the status quo and compromise the artifact integrity. Removable treatments can potentially avoid erosion of the artifact integrity.
Microgel
particles have emerged in the past few years as a favorite
model system for fundamental science and for innovative applications
ranging from the industrial to biomedical fields. Despite their potentialities,
no works so far have focused on the application of microgels for cultural
heritage preservation. Here we show their first use for this purpose,
focusing on wet paper cleaning. Exploiting their retentive properties,
microgels are able to clean paper, ensuring more controlled water
release from the gel matrix, in analogy to their macroscopic counterpart,
i.e., hydrogels. However, differently from these, the reduced size
of microgels makes them suitable to efficiently penetrate in the porous
structure of the paper and to easily adapt to the irregular surfaces
of the artifacts. To test their cleaning abilities, we prepare microgels
made of Gellan gum, a natural and widespread material already used
as a hydrogel for paper cleaning, and apply them to modern and ancient
paper samples. Combining several diagnostic methods, we show that
microgels performances in the removal of cellulose degradation byproducts
for ancient samples are superior to commonly employed hydrogels and
water bath treatments. This is due to the composition and morphology
of ancient paper, which facilitates microgels penetration. For modern
paper cleaning, performances are at least comparable to the other
methods. In all cases, the application of microgels takes place on
a time scale of a few minutes, opening the way for widespread use
as a rapid and efficient cleaning protocol.
The purpose of this study was to correlate the chemical composition of four commercial concentrated glycerine macerates (C-GMs), produced through the same extraction method, with their in vitro antimicrobial, antioxidant, and immunomodulatory properties, in order to evaluate their potential for healing upper airway diseases. C-GMs of Carpinus betulus (CB), Ficus carica (FC), Alnus glutinosa (AG) and Ribes nigrum (RN) were studied. The quality was evaluated using HPLC and IM-SPME/GC-MS systems; anti-oxidant and anti-microbial activities were assessed by the respective DPPH test, and micro-broth dilution test performed against 10 strains of Streptococcus pyogenes and 10 probiotic strains. ELISA and MTT tests were used to assess the immunomodulatory activity and the cytotoxicity of C-GMs, respectively. A significant correlation was found between the number of active compounds and the in vitro C-GMs effectiveness. Furthermore, the C-GMs of AG showed the best anti-microbial activity on pathological strains and, together with CB, the best anti-oxidant activity. The ELISA test exhibited a good immunomodulatory activity of RN. In vitro data support the integrated use of C-GMs of CB, AG, and RN in presence of airway diseases, and highlight the importance of standard procedures in cultivation, harvest and post-harvest treatments, as a premise for C-GMs with consistent characteristics.
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