Cellulose Nanoparticles Extracted from Sugarcane Bagasse and Their Use in Biodegradable Recipients for Improving Physical Properties and Water Barrier of the Latter

The present work firstly aimed to obtain cellulose from sugarcane bagasse by using alkaline methods in pulping/delignifying and, at bleaching stages, using sodium chlorite, glacial acetic acid, and hydrogen peroxide, associated to NaOH/KOH. The process was carried out at temperatures varying from 55°C to 110°C, under magnetic stirring in various steps lasting from 2 h to 12 h. The yields of the two cellulose extracted, SCB24-Na-I and SCB24-Na-II, were 37% and 41%, respectively, from samples of ca. 15 g of the bagasse. Secondly, it is to extract nanoparticles from the obtained celluloses via acid hydrolysis (with 77% H2SO4) to lately be tested as reinforcement in biodegradable packagings. Both celluloses and their respective nanoparticles were characterized by several techniques, among them ATR-FTIR, DSC-TGA, XRD, SEM, and TEM. Despite that the yields of cellulose nanoparticles have been low, the 
preliminary studies of their use in biodegradable films coated on biodegradable pots were promising.


Part A: Methods for Characterizing Sugarcane Bagasses,
Extracting Celluloses Therefrom and Characterizing the Latter 1) Biomass Moisture Content Samples of 1 to 3 g in triplicate of sugarcane bagasse (SCB) were weighed on an electronic analytical balance Mettler-Toledo with 10 −4 precision, using aluminium foil molds as tare weights, and dried on a hot air circulating oven at 105˚C ± 5˚C for at least 3 h. Then, the dry samples were kept in a desiccator for subsequent weighing at room temperature and humidity (23˚C ± 2˚C and 68% ± 2%).
The percentage moisture content was calculated from the variation of the weight of the wet sample, according to Equation (1).
where %H is the percent water content in the biomass, m i and m f are the initial and final weights of the moist and dry biomass, respectively. The final results were taken as the arithmetic mean of the moisture contents of the samples tested and including the standard deviations.

2) Biomass Ash Content
Ca. 2 g/sample of SCB in duplicate was weighed in porcelain crucibles (tare weights) on the same electronic analytical balance cited in "Biomass moisture content". After weighing the biomass samples, their burning was processed in a muffle furnace-Fanem electric oven of 220 V, Mod. 412, up to 1200˚C, Brazil-at 600˚C for 2 h. After removed cautiously from the muffle, with appropriated nippers, the samples were transferred to a dissicator, where they were kept for acclimating and subsequent weighing at room temperature and humidity conditions (23˚C ± 2˚C and 68% ± 2%). Ash content was calculated according to Equation (2).
% 100 where %A is the percent ash content, m i and m f are weights of SCB and of its incineration residue, respectively. The final results were taken as the arithmetic mean of the ash contents of the samples tested and including the standard deviations.

3) Dewaxing of Sugarcane Bagasse (SCB48)
A Soxhlet extractor set was utilized in this experiment, mounted in a fume hood. Ca. 2 g of SCB48/experiment was packed into a cellulose thimble (Soxfit from Labynth, Diadema-SP, Brazil) and placed in the appropriated compartment of the set; the reflux balloon was filled with 300 mL of a toluene-ethanol solution (2:1, v/v, respectively), and the system was heated and screening, the bagasse residue in each sieve was weighed, and its percentage distribution of particle/fibre sizes was estimated.

Washing and Drying of the Bagasses Selected Granulometrically
The bagasses with granulometries (in mesh) chosen subjectively for the subsequent tests were coded as SCB48 and SCB24, that is, those retained on 48-and 24-mesh sieves, respectively. Washing was made using tap water at 55˚C for 5 times on average, with the aid of the metal sieve of 80 mesh until the filtrate became transparent and practically colorless. The washing purpose was to remove saccharides/polysaccharides and other water-soluble components. The bagasses were then drained into the sieve itself; thereafter, they were transferred to teflon-coated aluminium trays for drying in a circulating hot air oven at 105˚C ± 5˚C for at least 12 h.
Next, addition of 0.0015 g of anthraquinone dissolved in 20 mL of absolute ethanol, 100 mL of 20% NaOH aqueous solution (m/v). The Erlenmeyer flask containing the whole mixture was placed on an electric heating steel plate with temperature regulation, kept under magnetic agitation and temperature regulated to 90˚C -100˚C. The Erlenmeyer flask mouth was tightly sealed with a PVC transparent film, followed by an aluminum foil reinforcement. The mixture was cooked for 24 h. Afterwards, the material was cooled at room temperature and filtered-with the aid of a vacuum pump-in a previously weighed appropriate Whatman filter and using a Büchner funnel coupled to a 600 mL Kitasato.
The filtrate was collected in the Kitasato. The washing of the residue was done with distilled water for several times until the filtrate reached the neutral pH or slightly below the neutral one (between 6 and 7, measurements by pH strips, Macherey-Nagel brand). The residue with the paper filter was placed on glass Petri dishes for drying in a circulating hot air oven at 70˚C for at least 2 h. After acclimating at 23˚C and 65% humidity, it was weighed to quantify the yield of Partial adaptations of the processes of delignifying and delignifying/bleaching were based on the works of Rocha, Sivério and their coworkers, and are summed up as described in Scheme 1 and Scheme 2, respectively.
Celluloses Extracted from Sugarcane Bagasse (SCB24) in an Optimized Process SCB24 without having been previously submitted to Sohxlet extraction was used as starting bagasse. Approx. 50 g of the bagasse were immersed in tap water in a kettle, which was heated on an electric plate until the boiling of the system.
After 10 min of boiling, the bagasse was cooled at room temperature and manually pressed in a 80 mesh metal sieve, washed with tap water for four consecutive times, always manually pressed after each washing operation to remove excess water. Then, the lignocellulosic mass was dried in a hot air circulating oven at 70˚C during 12 h. Scheme 1. Sugarcane bagasse (SCB48) delignification [30].  [31].
Two portions of 15 g were removed from the dry biomass for the pulping and bleaching experiments. Their pulping/delignification was carried out using for each sample: 300 mL of 5% NaOH (m/v), 50 mL of absolute ethanol, <0.002 g of anthraquinone in a 600 mL glass beaker or erlenmeyer provided of magnetic stirrer. The suspensions were covered with PVC plastic films and aluminium foils, then placed on hot steel plates, where they were kept under stirring at 90˚C -100˚C for 6 h. Thereafter, they were cooled at room temperature, submitted to vacuum filtrations, whose residues were washed with distilled water several times, fallowed by filtration after each washing until the filtrate reached a pH ca.

7.
Next, each residue from pulping/delignification was treated with a mixture of 150 mL of aqueous sodium chlorite at 1.7% (m/v) and 150 mL of aqueous where I 002 or totaI I represents the maximum intensity at 2θ = 23˚, crystalline region of cellulose, and I am at 2θ = 18˚, amorphous region of cellulose.

10) Scanning Electron Microscopy (SEM)
The samples of bagasse (SCB) and celluloses thereof were tested without a previous metallic sputtering (gold, palladium, others) on a SEM Jeol Neoscope JCM 5000 instrument with a conventional tungsten filament cannon, fixed acceleration voltages of 15, 10, and 5 kV, a maximum magnification of ×40,000, and observation at high and low vacuum (30 Pa).
Note: Origin 8 program was used in the processing of the results obtained in the laboratory were taken by the camera of a Samsung mobile phone.

Part B: Methods for Obtaining Cellulose Nanoparticles, Their
Characterization and Application as Coating on Biodegradable Recipients Two types of cellulose were used (Figure 2), both extracted from sugarcane bagasse from the same power plant, but differing in treatment-with and without KOH aqueous solution of the cellulose filtration residue, after the second bleaching. CBC1 was denominated the sugarcane bagasse cellulose with KOH-treated residue, originally named as SCB24-Na-I, and CBC2, the sugarcane bagasse cellulose without KOH-treated residue, originally named as SCB24-Na-II.

Production of Nanoparticles of Cellulose (NPCs)
In order to obtain the cellulose nanoparticles (NPCs), hydrolysis was carried out using sulfuric acid (SA) in accordance with the methodology adapted from Michael Ioelovich (2012) [28]. To prepare the NPCs the following treatment conditions were used for the acid hydrolysis: SA concentration at about 77% (m/v); ratio of acid volume/cellulose mass = 9; temperature between 45˚C and 55˚C; and 60 min time of reaction. The hydrolysis procedures were quenched by adding ice-cold distilled water into each reaction mixture. The cellulose sediments of the formed suspensions were separated from the liquid phase by various centrifugations (rotational speed of 6500 rpm for 25 min in a Quimis tube centrifuge) and subsequent washes with distilled water and addition of 5% potassium carbonate aqueous solution (m/v) separately until the suspensions reached the neutrality (pH ≈ 7.0). The pH measurements were checked by means of pH tapes at each washing/centrifugation of the suspensions. Their dry powders (the expected NPCs) were obtained by lyophilization in a vertical lyophilizer containing 6 glass bottles from Solab Equipamentos de Laboratório Ltda., thus allowing to calculate the yield (R) of the different suspensions, that is, R = (m powder after liophilization × 100)/m initial of cellulose . CBC1 CBC2 Figure 2. Visual aspect of the two types of sugarcane bagasse cellulose: CBC1 (with KOH-treated residue, originally named as SCB24-Na-I) and CBC2 (without KOH-treated residue, originally named as SCB-Na-II), used separately to obtain their nanoparticles. CBC = sugarcane bagasse cellulose. Materials Sciences and Applications The water dispersions of the nanoparticles were evaporated in a vacuum system at 80˚C for 24 h, then washed with distilled water and finally homogenized in a MaxiClean-1400 sonicator at 40 kHz for 30 min, resulting in different suspensions of nanocellulose. For the production of NPCs, preliminarily only 2.0 g of each CBC was used, due to the small amounts obtained in the extraction process; the remainders of the samples were used to obtain their NPCs to be incorporated in biodegradable recipients (plants pots made of sugarcane bagasse) separately. To do this, both celluloses were cut into small pieces (as much as possible) with the help of a pair of scissors, before starting the reactions, as shown in Figure 3.
The hydrolysis for each CBC was performed under the same treatment conditions: SA (acid sulfuric acid) concentration at about 77% (m/v); ratio of acid volume/cellulose mass = 9; temperatures between 45˚C and 55˚C; reaction time of 60 min, resulting, therefore, in two different suspensions: SCBC1 and SCBC2, shown in Figure 3.
The two suspensions obtained had the same visual characteristics between themselves, being apparently homogeneous and of dark color (black) soon after the hydrolysis ceased (Figure 4(a)), and heterogeneous after 24 hours, with sedimented cellulose particles and light yellow supernatants (Figure 4(b)).
After neutralization by washes with distilled water and KHCO 3 aqueous solution until pH ≈ 7.0-18 washes and centrifugations for SCBC1 and 24 washes and centrifugations for SCBC2-parts of the obtained suspensions were sent to transmission electron microscopy (TEM), and the remaining ones lyophilized for subsequent calculation of yield and scanning electron microscopy (SEM) analysis.

1) Transmission Electron Microscopy (TEM) of Cellulose Nanoparticles' Suspensions
Both samples (SCBC1 and SCBC2) suspended in distilled water were analyzed by transmission electron microscopy (TEM) at the Materials Science and Technology Center of IPEN, using an electronic microscope, JEOL brand and JEM-2100 model. A small portion of both samples (in suspension) were analyzed by energy dispersive spectroscopy (EDS) at 5, 20 and 50 nm scales.
2) Yields (R) of Cellulose Nanoparticles' Suspensions The yields (R) of the different cellulose nanoparticles' suspensions were calculated by the Equation (4): R = (m powder after liophilization × 100)/m initial of cellulose where m is the mass in g on dry basis.
3) Scanning Electron Microscopy (SEM) of Cellulose Nanoparticles' Suspensions Both lyophilized samples (SCBC1 and SCBC2), dry, were analyzed by SEM at the Lasers and Applications Center of IPEN, using the Tabletop SEM equipment of the HITACHI brand and model TM3000. Small portions of both samples were analyzed by the program's "Analy" (AL) system, with increases of 500 and 1000 times.  The production of new nanoparticles of the CBC1 and CBC2 celluloses to be brushed on biodegradable recipients occurred in the same way described pre-  Figure   5.

SCBC1 SCBC2
After the hydrolysis ceased ( Figure 5(a)), the two suspensions obtained had the same visual characteristics compared each other, being apparently homogeneous and of dark (black) coloration, but after 24 hours ( Figure 5(b)), the two suspensions showed some differences between each other, although not all of the cellulose particles sedimented on the bottom of the beakers, a fact that was further evidenced, in much smaller proportions, when NPCs were produced from hydrolyses of 2.0 g of each CBC (as shown in the SCBCs of Figure 6). The minutes, and subsequent manual shaking for another 5 minutes. Thus, two gels were obtained, which we named as "F-CBC1" containing NPCs formed from CBC1 (KOH-treated cellulose) and "F-CBC2" containing NPCs formed from CBC2 (KOH-untreated cellulose). For comparison effect of both substances, a standard film-forming suspension was also made; it means, without NPCs, using equal amounts of starch, glycerin and water, denoted only by "F". Figure 7 shows the three produced gels.
The three film-forming suspensions obtained, all in exactly 20 minutes under constant stirring and heating on electric steel plates, apparently presented the same viscosity, and were characterized as "gels". From Figure 7, it can be seen that the addition of the CBC1 and CBC2 NPCs to the mixtures to form their film-forming suspensions resulted in dark gels, unlike that with no NPC ("F" suspension), as expected due to the purplish color of NPCs produced.
Parts of these three film-forming suspensions (gels) produced were brushed as a thin layer on the inside of 30 biodegradable recipients-10 recipients brushed with each gel-and the remainder distributed in a total of 36 polystyrene Petri dishes with internal diameter of 5.8 cm. Initially, 4.0 g of each gel was weighed into 6 Petri dishes and subsequently 3.0 g of each gel into 6 additional Petri dishes (in order to fill the entire dish/plate) with the intention of forming the thinnest films as possible to resemble those who would eventually form inside the biodegradable recipients. All Petri dishes and recipients containing the different film-forming suspensions were placed in a drying oven at 60˚C ± 2˚C, with air circulation, for 4 hours. Figure 8 shows the 30 internally coated recipients   The different formed films were kept in the fume hood of the Polymers Laboratory of the CQMA/IPEN, at room temperature and relative humidity (respectively, 20˚C to 25˚C and 76% to 88%) for 48 hours until they absorbed a little moisture, purposely, to facilitate their detachments from their respective Petri dishes. This procedure was done because, as soon as the dishes were removed from the oven, the obtained films showed to be a little brittle, and their removals probably would be very difficult.

5) Water Absorption by Biodegradable Recipients with and without Sugarcane Bagasse NPCs
It is worth noting that, for the accomplishment of this experiment, the recipients (pots for growing seedlings) without holes in their bottoms were used to hinder the water drain. Five recipients (without hole) for each type of applied inner coating (F, F-CBC1 and F-CBC2) were weighed, and 200 mL of water were added therein for 60 seconds at room temperature. After this period, the water was discarded and its excess removed until no more drops of water dripped from inside the recipients, which were weighed again. Finally, the mean values of

6) Moisture Absorption by Biodegradable Recipients with and without
Sugarcane Bagasse NPCs The moisture content of recipients without coating and those coated with and without NPCs, kept in the fume hood of the CQMA/IPEN Polymers Laboratory, throughout the days, without controlled temperature and humidity, was calculated as a percentage of the initial mass of the packing. The weighing of the recipients was done with a digital balance, at time zero (when they were removed from the drying oven of their respective films) and then every seven days. For each type of coating (with and without NPCs), five recipients were used, calculating the moisture content averages. The same procedure was done for recipients without coating (SEM F) for comparison purposes. It is worth remembering that this assay was done for only 14 days due to the short time remaining for submission this report (Fundep deadline).

7) Crotalaria Plantation in Biodegradable Recipients with and without
Sugarcane Bagasse NPCs The internally coated recipients with film-formig suspensions (gels) with and without sugarcane bagasse NPCs and those without coating (for comparison purposes) were used for planting crotalaria (Crotalaria juncea), in order to verify the influence of these recipients on the plant development and their physical integrity during the nursery phase-it means, during the germination and growth of the seedlings to further be transplanted into the field without removing them from the recipients-since they are biodegradable and compostable. It is noteworthy that, unfortunately, it will not be possible to show the transplantation phase in this report due to the limited time for submission of this work. For the same reason, the results of the plants' development and the recipients' integrity in the crotalaria planting will be presented only during the first fourteen days of seedling.
For planting, five recipients of each type of studied coating in this project were used (with and without the sugarcane bagasse NPCs), as well as the same amount used for those without coating. All recipients were filled to the brim with peat "Tropstrato Florestal", from Vida Verde Indústria e Comércio de Insumos Orgânicos Ltda., as shown in Figure 9, and in each of them four crotalaria seeds ( Figure 9) were buried superficially.
Among the many seed options available to plant and taking into account the short time remaining for submission this report (deadline), we chose for Crotalaria juncea because, through experiments carried out before this SIBRATECNANO project, our researchers' team verified that the crotalaria germination and the plant development occur very quickly and efficiently in greenhouse, and such seeds ( Figure    such analyzes (for this report) no longer 14th day of sowing, according to the reason already explained previously. The averages for each of these measurements and in each type of recipient used in this test were estimated before transplanting the seedlings into the field. It is worth mentioning that it was decided to make the first stalk diameter measures just 15 days after the beginning of plantation, because before that, the seedlings stalks were still very fragile.

9) Integrity of the Recipients with and without Sugarcane Bagasse NPCs along the Plant Development
Because they are made of biodegradable materials from renewable natural sources (sugarcane bagasse and cassava starch), the recipients are very sensitive to moisture and water (from irrigation), thus causing deformations on their edges, walls and bottoms. Such events lead them to softening, cracking, and they subsequently rupture as time goes by. Hence, the objectives of studying the incorporation of sugarcane bagasse NPCs (CBC1 and CBC2) into these recipients The integrity of the uncoated recipients and those coated by the different film-forming suspensions (with and without the sugarcane bagasse NPCs) were analyzed weekly, from the day of sowing (zero time) until the 14th day of planting, and the reason for the short test period was previously explained in this report. The study was based on the softening and/or cracking 1) of the edges, 2) walls (body), and 3) bottoms of the recipients, being numerically evaluated from 3 to 0, where the recipients numbered: 3 = good (integers, without any modification); 2 = softened and/or cracked; 1 = very softened and/or very cracked; and 0 = broken/dismantled.

Biomass Moisture Content
Sugarcane bagasse, originally received from the supplier with moisture ca. 50%, after dried in the sun for 8 h at ca. 30˚C, showed 27.22% ± 0.78% moisture from samples tested in triplicate. After dried, ground by the miller equipped with a knife system, its moisture dropped to 15.54 ± 0.03 from another triplicate of samples evaluated, fact already explained in "Main raw material".

Original Biomass Ash Content
The results of ash content were: 2.42% ± 0.81% for SCB and 1.02% ± 0.03% for WP. In the case of sugarcane bagasse, Pandey et al. (2000) [33] cite their chemical composition with 2.4% ash content, and other authors found values close or well above, for example, 5.4% [34]. Figure 11 shows ashes of incinerated sugarcane bagasse (SCB) and wood powder (WP) from a furniture industry (as reference).
The ash colors of the wood powder and sugarcane bagasse were quite different each other: darkgrey and reddish-grey, respectively ( Figure 11). It probably is due to formation of different metal oxides throughout incineration of the materials, and those were not identified. Here it is worth mentioning that their coloration may depend on lots of factors, such as, soil nature and contaminants, fertilizers in the plant cultivation, metals absorbed by the plant in the metabolism, the crop season, and the storage conditions of the lignocellulosic residues in sugar/alcohol industries. For example, the bagasse we have used in production of biodegradable tubes and vases (for agriculture), and trays (for food packaging) at Bio & Green comes with various color shades: from yellowish to light brown.
Note: On following of the tests, the wood powder (WP), originated from a furniture factory, contained crosslinked resins as numerous formica particles of difficult removal from the wood (maybe some species of pinus or eucalyptus).
Owing to that, one gave up to continue its tests for comparison with those on sugarcane bagasse, except for the XRD test. This type of sieving process, done manually and prone to reasonable losses in manipulation (for instance, as wood dusts in the air), probably is less accurate than that done by using an electrical system with an appropriate vibrator, whose time and intensity of the vibrations can be programmed. One must still consider the irregularity of the material in terms of fiber/particle sizes, making difficult to obtain high amounts of low-sized fibers/particles from a unique batch. In the choice of lignocellulosic materials for subsequent tests, SCB48 (sieving residue on the 48 mesh sieve) was subjectively chosen. Throughout the experiments, SCB24 (residue on the 24 mesh sieve) also was tested in some characterization items and had a performance practically equal to that of SCB48.    [38]. One must take in account that the yield differences of extractables come from the variety of solvents, processing duration times, and different temperatures utilized in this test, whose parameters depend on the researcher choice without following rigid patterns.      The exemplification in Figure 13 refers to the first of the last three experiments mentioned in Table 2, showing a bleaching stage of the raw cellulose. For a partial discussion in Table 2 and Figure 13, let us comment, for example, the preliminary pulping/delignification, where there were two steps (**), on Jan. 9,  previously submitted to a Soxhlet extraction (SCB48sox). In the first step, pulping/delignification with an aqueous 20% (m/v) NaOH solution at 90˚C -100˚C for 6 h. Its yield was 1.72 g of earthy yellow SCB48sox (33.92% in raw cellulose obtained from the original sample). In the second step, a bleaching of SCB48sox

Phase 1: Preliminary Pulping/Delignification and Bleaching of
with an aqueous solution of GAA-NaClO 2 at ca. 80˚C for 12 h afforded 1.36 g of earthy yellow color SCB48sox, probably owing to still small parcels of lignin remaining in the sample. This resulting sample was named as SCB48-Na for simplicity, whose photo is exhibited in Figure 13.
In continuation, after the first bleaching of SCB48-Na sample, its color practically did not change, in other words, it remained earthy yellow like the original one only delignified. Yield: 1.36 g of SCB48-Na after an expressive mass loss: 20.93% based on the 1.72 g sample. Thus, the total cellulose yield, relative to the original sample of ca. 4 g of bagasse, was ca. 34%. Therefore, this event discouraged us to attempt a second bleaching of the sample. For more detailed understanding of the two stages, Table 2 displays the pulping/delignification and bleaching data of five experiments with SCB samples.
In these preliminary studies, one noted that the use of Soxhlet-purified bagasse did not increase the bleaching level of the raw cellulose obtained. For a work aiming to obtain expressive amounts of cellulose for tests in semi-industrial or industrial scale, such a process practically would become unviable by cost, besides being hazardous to the environment.

A Partial Adaptation of Sugarcane Bagasse Delignification Based on the Work of Rocha et al. (2014) [31]
Along the pulping/delignification process, distilled water was added to the suspension: 50 mL, 50 mL, 100 mL, and 50 ml after 1 h, 2 h, 4 h, and 6 h, respectively, in order to compensate water losses by evaporation. The result was a dry lignocellulosic residue with dark brown color, that was discarded. For this reason, the NaOH concentration was increased from 0.8% to 5% (m/v), aiming at obtaining a lighter color of the raw cellulose. Thus, a new experiment was run with 5% NaOH, using ca. 8 g of SCB48 at the same conditions applied to the first pulping/delignification. The raw cellulose obtained showed a grayish-white color with ca. 53% yield ( in an Optimized Process At this stage, celluloses were extracted from sugarcane bagasse following the scripts presented in Table 3 and Table 4.  As starting bagasse, SCB24 was used without having been previously submitted to Sohxlet extraction. Approx. 50 g of this bagasse was immersed in tap water inside a kettle, which was heated to boiling of the system on an electrical heating steel plate. After 10 min boiling, the bagasse was cooled at room temperature and manually pressed in a 80 mesh metal sieve, washed with tap water for four consecutive times, always pressed after each washing operation to remove water excess. Then, the lignocellulosic mass was dried in a hot air circulating oven at 70˚C for 12 h. After cooled to room temperature, two portions of 15 g from the dry mass were removed for the pulping and bleaching experiments. Table 3 and  Table 4 summarize the data and results of delignification/pulping and bleaching processes. Delignification/pulping was carried out using aqueous NaOH-anthraquinone solution (Table 3(a)). Four bleachings were done at this stage (Table 3(b)), using for that blends of two aqueous solutions, 125 -150 mL of sodium chlorite at 1.7% (m/v) and 125 -150 mL of NaOH-GAA at 90˚C -100˚C for 4 h per sample each time, followed by several vacuum filtrations, washings with distilled water, pH adjustments. Then, four new bleachings were performed with 300 mL of aqueous solution containing NaOH and H 2 O 2 at 55˚C -60˚C for 2 h per sample each time (Table 4(a)). After each new bleaching, several vacuum filtrations, followed by washings with distilled water, were effected on the cellulosic residues until the filtrate reached a pH ca. 7. Next, final drying of the last residues in a hot air circulating oven at 70˚C for 24 h.
Both celluloses extracted from the SCB24 showed white staining ( Figure 14) but slightly more pronounced for SCB24-Na-I. The cellulose sugarcane bagasse yield was 37.06% for SCB24-Na-I and 41.31% for SCB24-Na-II (Table 4). They were considered promising for preliminary extraction of nanocelluloses therefrom.    [48]. Regarding the celluloses extracted from sugarcane bagasse-SCB24-Na-I and BCA-Na-II-CHN tests were not performed. Table 6 sums up absorption ranges, functional groups and attributions of the three main lignocellulosic components of sugarcane bagasse (SCB48 and SCB24).

Attenuated Total Reflection Fourier Infrared Spectroscopy (ATR-FTIR)
It also can help us deal with the interpretation of ATR-FTIR spectra of the raw celluloses (SCB48-Na, SCB24-Na-I, SCB24Na-II) obtained. Figure 15 shows the ATR-FTIR spectra of SCB48 and that of the raw cellulose extracted from this after treatments of the bagasse with an aqueous solution of sodium hydroxide containing a minimal parcel of anthraquinone for the deligni-

Thermal Analysis (TA): Differential Scanning Calorimetry (DSC) and Thermogravimetric Analysis (TGA) Sugarcane Bagasse (SCB24 and SCB48)
The endothermic peaks recorded from ambient temperature to 116˚C and 156˚C refer to the elimination of water retained in the bagasses SCB48 and SCB24- Figure 17(a) and Figure 17(b), respectively-linked to lignocellulosic components, chiefly to cellulose. Since the bagasse is formed by a complex mixture of components, the interpretation of DSC curves is not an easy task. The DSC measurements show, for example, that, even warming the sample of a pulp up to 170˚C, one cannot obtain it absolutely dry [51]. Two more important events were observed: an endothermic one in the range of 290˚C -355˚C due to the decomposition of cellulose and an exothermic one around 375˚C, possibly originated from the crystallization of cellulose.
Concerning the thermogravimetric analysis, Figure 18 shows the results of both SCBs.
The profiles of the TG/DTG curves- Figure 18(a) and Figure 18 [22]. The initial endothermy in the first stage of mass loss, which occurs in all two cases- Figure 18(a) and Figure 18(b)-at a temperature much lower than 110˚C up to ca. 120˚C, means the loss of moisture due to the evaporation of free water and that of low-molecular-weight compounds as well as elimination of water from intermolecular hydrogen bonds in biomasses.
In the second and third stages of mass loss, it occurs between 214˚C and 375˚C,  [53] for both bagasses. Following, two exothermic degradation peaks at 329˚C and 339˚C for SCB48 and SCB24, respectively. Possibly it is due to cellulose degradation (TG up to 400˚C). In the fourth stage, above 375˚C, any peak arising may refer to lignin degradation, which is quite complex, also involving more stages at temperatures below 375˚C [54]. All these peaks were revealed by the first derivative of TG. The differences are minimal between the profiles of the curves, indicating that they may probably originate from differences in sample quantities and not uniformity of the particle size/fibers of the biomass, in addition to impurities inherent to them.
About the the DSC of both celluloses, Figure 19 shows their profiles.
Two endothermic events were recorded in both celluloses, one with peaks at 142˚C and 160˚C, caused by evaporation of the water from room temperature to 160˚C or to enthalpy of dehydration, already explained from the results in Figure 17. The second endothermic peaks at 350˚C and 352˚C refer to decomposition of the cellulose. An exothermic event with peaks at 369˚C and 374˚C, possibly originated from the crystallization or enthalpy of cellulose crystallization [55]. Such peaks at the respective temperatures herein mentioned are depicted in Figure 19(a) and Figure 19 The results of TG/DTG were close to those described by Mandal and Chakrabarty (2011) [22] and Liu et al. (2006) [50] on tests of celluloses from sugarcane bagasse, noting that the decomposition of cellulose occurs in two exothermic stages in a range of 320˚C -375˚C. At 341˚C, mass losses were 95% for SCB24-Na-I and 87% for BCA-Na-II (curve profiles in Figure 20).

X-Ray Diffractometry (XRD) of the Sugarcane Bagasses and Celluloses Extracted Therefrom
The results from the X-ray diffractometry of SCB48 and WP24, as well as those of the celluloses extracted (SCB-Na-I and SCB-Na-II) from SCB24, were ob- where I 002 or I total represents the maximum intensity at 2θ = 23˚, the cellulose crystalline region, and I am at 2θ = 18˚, the intensity of the cellulose amorphous region. Some essential measurement data are in Table 7 and Table 8 (3), for the native celluloses of SCB48 and WP24 were ca. 56% and ca. 61%, respectively (inferred from Table 7 and Figure 21).     Such peaks of I am and I total considered in the CI calculations may vary around 16˚ and 22˚, respectively, in several publications [16] [56] [57]. The degrees of crystallinity, estimated based on Equation (3) for the celluloses extracted from sugarcane bagasse-BCA24-Na-I and BCA24-Na-II-were ca. 69% and ca. 68%, respectively (inferred from Table 8 and Figure 22). The profiles of both celluloses are very resembling each other.

Part B: Obtaining of Cellulose Nanoparticles, Their Characterization and Application as Coating on Biodegradable Recipients
Once neutrality was reached, after numerous washes with distilled water and centrifugations, a curious phenomenon was observed visually (with the naked eye) between samples of the SCBC1 and SCBC2 suspensions arranged separately in two Falcon tubes (Figure 25). After a slight manual shaking of these tubes, most of all the particles of the SCBC suspensions quickly settled-few particles remained dispersed in the suspensions SCBC1 and SCBC2 as supernatants. This phenomenon was probably due to a lowering of the colloidal stability of the particles and nanoparticles of cellulose in the dilute suspensions (supernatants) after shaking, tending to form larger agglomerates, which promptly precipitate.

Transmission Electron Microscopy (TEM) of Cellulose Nanoparticles' Suspensions
The images of the SCBC1 and SCBC2 suspensions obtained by TEM are shown in Figure 26 and Figure 27.

Yields (R) of Cellulose Nanoparticles' Suspensions
The yield of the SCBC1 and SCBC2 suspensions, based on 2.0 g of cellulose bagasse, calculated after their lyophilization, corresponded, respectively, to 9.6% and 12.0%, showing that the use of the different types of sugarcane bagasse cellulose (with and without KOH treatment) practically did not influence the yield of their nanoparticles, that is, a difference of only 2.4% between them.   and SCBC2 (2.4%) initially described. When comparing these two yields with those obtained from 2.0 g of both CBCs (SCBC1: 9.6% and SCBC2: 12.0%), it can be said that there was no significant yield increase by using 7.0 g of each CBC, but maintaining the same solid/liquid ratio.

Scanning Electron Microscopy (SEM) of Cellulose Nanoparticles
The images of the fragments (powders) resulting from the lyophilization of the SCBC1 and SCBC2 suspensions, obtained by SEM, are shown in Figure 28 and Figure 29. TEM and SEM analyses of the different cellulose particles from 7.0 g samples, as well as their suspensions in distilled water obtained after neutrality of SCBC1A and SCBC2A, were not performed once their nano-and microstructural characterizations have already been shown previously (subitems 3.2.1 and 3.2.3 of this work), when the NPCs (powder and suspensions) were produced from 2.0 g of the same CBCs studied in the project (Figures 26-29).

Brush Application of Cellulose Nanoparticles from Sugarcane
Bagasse on Biodegradable Recipients The thin layer of the different film-forming suspensions (gels) brushed on the biodegradable recipients selected for tests, after drying in the oven, provided some brightness in their internal parts, when compared to the recipients uncoated-these named by "SEM F". In addition, the application of the F-CBC1 and F-CBC2 gels caused the cellulose particles to be clearly visible in the inner of the recipients, evidenced by small purplish spots (and in greater quantity when utilizing CBC2), as well as in the films formed in the Petri dishes. Figures 30-32 show these details in some of the recipients and films, respectively. Figure 33 shows some of the films formed from 3.0 g and 4.0 g of the film-forming suspensions (gels), removed from their Petri dishes.
In the F-CBC1 and F-CBC2 films of Figure 32 and Figure 33, it can be seen that those containing 4.0 g of their respective film-forming suspensions (gels), the NPCs became more evident, in greater quantity and more concentrated in the center of the Petri dishes ( Figure 32) comparing to the films formed with 3.0    Table 10 shows the average thickness (in mm) of each film formed from 3.0 and 4.0 g of their respective film-forming suspensions (gels), which were measured using a Digimess electronic micrometer, from 0.001 to 25 mm accuracy. The incorporation of sugarcane bagasse NPCs into film-forming suspensions increased the thickness of the formed films, as expected (due to the presence of both nonsolubilized cellulose particles), especially when untreated sugarcane bagasse (CBC2) NPCs were added, as these become more concentrated and in greater quantity in the dried suspensions. Therefore, it can be said that the thinnest films were those produced by suspension without NPCs (F), while thicker films were formed by suspensions containing NPCs (F-CBC1 and F-CBC2), being those produced with untreated sugarcane bagasse NPCs (F-CBC2) the thickest ones. It is still noted in Table 9 that as higher the amount of suspension, obviously, higher the film thickness.
The recipients internally coated by a thin and dried layer of the three gel types, after also remaining purposely 48 hours in the fume hood of the Polymers Laboratory of the CQMA/IPEN (for the same reason mentioned above), at room temperature and relative humidity, could not have their films detached from their walls, and, consequently, it was not possible to measure their thicknesses. This impossibility most probably occurred due to the very small amount of film-forming suspensions brushed on the inner part of the recipients and perhaps also due to the adhesion of these very thin layers of the different gels to the porous walls of the recipients, thus making it difficult to form films and their consequent detachments. Despite the nonformation of "palpable" films, and in order to at least quantify the different film-forming suspensions (gels) that were brushed internally on each recipient, it was decided to weigh such recipients after drying-since they had already been weighed prior to the application of their coatings-using a digital analytical balance, and thus calculating the average amounts of the different gels in them. Table 10 shows the average amounts (in g) of the different film-forming suspensions (gels) brushed on the recipients. It is worth noting that the values shown in the referred table represent approximated average quantities since such recipients possibly absorbed moisture after being removed from the oven and remaining in the laboratory fume hood for 48 hours without controlled temperature and relative humidity. Table 9. Average thickness of films produced from 3.0 and 4.0 g of each studied film-Forming suspension (Gel), after detachment of their respective petri dishes.  It can be seen from Table 10 that actually a very thin layer of each suspension (gel) was brushed on the inner part of the recipients, all of them corresponding to less than half a gram; there was no significant difference among them. As expected, the highest amounts were observed in the NPCs-coated recipients, especially when incorporating the untreated sugarcane bagasse cellulose (CBC2) particles. The difference of applied quantity in the recipients between that of gel without NPCs (F) and those of the gels with the sugarcane bagasse NPCs (F-CBC1 and F-CBC2) was approximately 0.1 g.
In order to verify the influence on the physical and water barrier properties of the recipients after coated with sugarcane bagasse NPCs, the pots were submitted to the tests of: 1) water absorption; 2) development of crotalaria plantation in them, and 3) integrity of the recipients with and without coatings (gels). Moisture absorption by recipients with and without coatings (gels) was also studied over 14 days-reduced and limited time due to the deadline for submission this work.

Water Absorption by Biodegradable Recipients with and without Sugarcane Bagasse NPCs
The results of water absorption by biodegradable recipients with and without sugarcane bagasse NPCs are presented in Table 11 and expressed in water absorption content (%).
The different coatings applied inside of the recipients significantly contributed to the reduction of water absorption. It can be said that, in general, the coatings reduced in almost half the water absorption by the recipients (when compared to the SEM F recipients), being those coated with film-forming suspensions containing NPCs (F-CBC1 and F-CBC2) the ones which less absorbed water, especially when using the CBC particles without residue treatment (CBC2). Figure 34 presents the results of moisture absorption by the different recipients, along the days, without controlled temperature and relative humidity, expressed in moisture content (%).

Crotalaria Plantation in Biodegradable Recipients with and without Sugarcane Bagasse NPCs
Crotalaria juncea is an annual spring-summer legume, growing very fast and vigorous, and its species produces the highest amount of biomass in the shortest time and, consequently, supplies nitrogen in greater quantity [64]. Crotalaria has its origins in India and Tropical Asia, and, interestingly, it helps to combat the mosquito that transmits dengue fever. Its beautiful yellow flowers attract the dragonflies, which need clean water to place their larvae. These larvae devour those of the Aedes aegypti mosquito and, after adults, the dragonflies also feed on the larvae of dengue main vector in Brazil [65].
Some of the crotalaria seeds of this study germinated in only three days of sowing, and on the fourth day of planting all recipients (without exception) already contained at least one of their sprouts (remembering that four seeds were planted in each vessel), as shown in Figure 35.    The average number of leaves of crotalaria was the same in the different reci-  Figure 39 shows only one curve in the graph, where in fact the curves are superimposed one another. The plants developed in both uncoated and coated with and without sugarcane bagasse NPCs presented 4 leaves on the seventh day and 6 leaves (two more) on the 14 th day after sowing; so there is no difference in the number of leaves between the recipients with and without coating of film-forming suspensions (with and without NPCs).
Integrity of the Recipients with and without Sugarcane Bagasse NPCs along the Plant Development As a reminder, the pots were qualitatively evaluated by assigning them numerical values from 3 to 0, where: 3 = good (integers, without any modification); 2 = softened and/or cracked; 1 = very softened and/or very cracked; and 0 = broken/dismantled. Figures 40-42 show the integrity of the edges, walls and bottoms, respectively, of the different recipients during the first 14 days of planting.

Bottom quality
Integrity of the Edges Figure 40 displays the profile of quality of the edges. Seven days after sowing, with the exception of the recipients coated with untreated sugarcane bagasse NPCs (F-CBC2 = blue bars), at least two of five recipients of each type in tests had their edges softened to level 2. On the seventh day, the edges of the five recipients coated with untreated sugarcane bagasse NPCs (F-CBC2 = blue bars) remained intact, with no modification, whereas practically all recipients without coating (4 of the 5 SEM F recipients = gray bars) had their edges softened to level 2. On the same day, three of the five recipients coated with no NPCs (F = red bars) and the same amount of those coated with treated sugarcane bagasse NPCs (F-CBC1 = green bars) did not show any changes in their edges. Fourteen days after sowing, all the five recipients coated without NPCs (F = red bars) had their edges softened to level 2-equal level of deformation was verified in: 4 recipients without film (SEM F = gray bars); 3 of the recipients coated with treated sugarcane bagasse NPCs (F-CBC1 = green bars); and 2 of those coated with untreated sugarcane bagasse NPCs (F-CBC2 = blue bars). Thus, in general terms, it can be said that, up to the present time, it means, in 14 days after crotalaria planting, the recipients which presented their most preserved edges were those coated with KOH-untreated sugarcane bagasse NPCs (F-CBC2 = blue bars), followed by those coated with treated sugarcane bagasse NPCs (F-CBC1 = green bars). In this same period, the recipients coated without NPCs (F = red bars) were the most damaged on their edges.
Integrity of the Walls In relation to the walls' integrity of the recipients in the crotalaria plantation ( Figure 41), it is verified that, seven days after sowing, the quantity of recipients with softened walls at level 2 was higher for those without coating (three of the five SEM F = gray bars), followed by recipients coated without NPCs and with treated sugarcane bagasse NPCs (two of five: F = red bars and F-CBC1 = green bars). On the same day, the recipients coated with KOH-untreated sugarcane bagasse NPCs (F-CBC2 = blue bars) did not show changes in their bodies. Seven days later, it means, on the 14th day of planting, the walls' conditions of practically all the previously analyzed recipients remained the same, except for one of the five recipients coated with untreated sugarcane bagasse NPCs (F-CBC2 = bars blue), which had its body slightly softened (at level 2). Thus, in general terms, it can be said that up to now, it means, in 14 days of crotalaria planting, the recipients which presented their most preserved walls were those coated with KOH-untreated sugarcane bagasse NPCs (F-CBC2 = blue bars), followed by those coated with KOH-treated sugarcane bagasse NPCs (F-CBC1 = green bars), and in the same amount of the latter, by those coated without NPCs (F = red bars). In this same period, the bodies of the recipients without film (SEM F = gray bars) were the most damaged.
Integrity of the Bottoms From Figure 42, it can be inferred that the bottoms were the recipient parts that most suffered changes in comparison to their other analyzed parts (edge and walls) in this experiment, in which practically all the recipients had their bottoms' quality fell to level 2 (soft), and even to level 1 (very soft), on the seventh day of the crotalaria plantation. Seven days after sowing, only one of the five recipients coated with KOH-untreated sugarcane bagasse NPCs (F-CBC2 = blue bars) kept its bottom intact, without any modification; however, on the 14th day of planting, this same recipient had its bottom softened at level 2 (soft), and it was the only change observed between the two days of this test analysis by the way. On the 7th and 14th days of planting, the number of softened recipients at level 2 (soft) was: 2 of the uncoated recipients (SEM F = gray bars); 3 of those coated without NPCs (F = red bars); and 3 of those coated with treated sugarcane bagasse NPCs (F-CBC1 = green bars), and the rest of the five recipients of each studied group were qualified at level 1 (very soft). Thus, in general terms, it can be said that up to now-it means, in 14 days of crotalaria planting-the recipients which presented their most preserved bottoms were those coated with KOH-untreated sugarcane bagasse NPCs (F-CBC2 = blue bars), followed by those coated with KOH-treated sugarcane bagasse NPCs (F-CBC1 = green bars) and, in equal quantity, the recipients coated without NPCs (F = red bars). In this same period, the bottoms of the recipients without film (SEM F = gray bars) were the most damaged.
In summary, the starch coatings somehow improved the resistance of the edges, walls, and bottoms of the recipients (data shown in Figures 38-40, respectively), along with the plantation development for 14 days, however with somewhat better results for those containing NPCs.

Conclusions
The pulping and bleaching of sugarcane bagasse based on the alkaline process involved numerous chemical treatments to achieve celluloses with a reasonable whiteness. From a selfcritical vision of the results, they were classified as raw celluloses.
Successive vacuum filtrations and washings with distilled water may lead to reasonable decreases in cellulose yields.
NaOH/KOH at concentrations above 4% (m/v), associated with temperatures of ca. 100˚C and cooking times above 2 h under mechanical or magnetic stirring, appeared to play the most important role in the bagasse delignification.
The celluloses extracted from the sugarcane bagasse (SCB24-Na-I and SCB24-Na-II with yields ca. 37% and ca. 41%, respectively) presented characteristics very close to each other, based on the results from their characterizations. Both products were considered promising in terms of coloration (acceptable whiteness) and future technological applications.
The acid hydrolysis conditions applied to the celluloses extracted from the sugarcane bagasse, with and without KOH treatment of their filtration residues during the extraction processes, allowed us to obtain their NPCs, represented in the TEM images by a mixture of fibrils and spheres, thus evidencing the formation of nanocellulose particles in a needle form.
The sugarcane bagasse NPCs incorporation, through thin layers of film-forming suspensions brushed inside of the biodegradable recipients, made the pots physically more resistant along with crotalaria growth-after their edges, walls and bottoms having been analyzed-not interfering in the good plant development (seedlings' heights and quantity of leaves). In addition, the sugarcane bagasse recipients coated with NPCs absorbed less water than those that were coated without nanoparticles, especially when compared to those without coating.
Although the sugarcane bagasse NPCs improved the physical and water barrier properties of the recipients, the time and water consumption during the washes and centrifugations of the suspensions (obtained after hydrolysis) until to achieve neutrality were exorbitant-mainly considering the very low amount of CBC used (7.0 g of each type)) and its very low yield.
The technique used for NPCs' production in this project for their later incorporation in the biodegradable recipients almost became impracticable in laboratory and probably, the same would occur at industrial levels, too, especially for a sustainable company. Thus, it still demands deeper studies in terms of the process time (very long) for obtaining the nanoparticles besides trying to increase their yields (low in this case) and lower the high cost of the whole process in general.