Short-Stranded Zein Fibers for Muscle Tissue Engineering in Alginate-Based Composite Hydrogels

Cultivated meat is a nascent technology that aims to create an environmentally and animal-friendly alternative to conventional meat. Producing skeletal muscle tissue in an animal-free system allowing for high levels of myofusion and maturation is important for the nutritional and sensorial value of cultivated meat. Alginate is an attractive biomaterial to support muscle formation as it is food-safe, sustainable and cheap and can be crosslinked using non-toxic methods. Although alginate can be functionalized to promote cell attachment, limitations in its mechanical properties, including form, viscosity, and stress relaxation, hinder the cellular capacity for myogenic differentiation and maturation in alginate-based hydrogels. Here, we show that the addition of electrospun short-stranded zein fibers increased hydrogel degradation, resulting in faster compaction, improved cell–gel interaction, and enhanced alignment of bovine muscle precursor cells. We conclude that fiber-hydrogel composites are a promising approach to support optimal formation of 3D constructs, by improving tissue stability and thus prolonging culture duration. Together, this improves muscle-related protein content by facilitating myogenic differentiation and priming muscle organoids for maturation.


Introduction
Cultivated meat (also known as 'cultured meat') is an evolving field that aims to produce meat products without the adverse environmental and animal welfare implications inherent to conventional meat production [1][2][3] by leveraging the in vitro proliferation and differentiation of stem cells.Although substantial progress has been made in recent years, including the development of animal-component-free processes [4][5][6][7][8], several major challenges are still being addressed to facilitate the mass commercialization of these technologies [3].
A central premise of muscle tissue engineering for cultivated meat is the emulation of the sensory and nutritional properties of skeletal muscle, which is contingent on the myogenic differentiation of muscle precursors (such as myoblasts) to form myotubes in three-dimensional tissue constructs.Subsequent maturation, marked by the increased biosynthesis of muscle-related structural proteins, might help mimic the characteristic taste, texture, mouthfeel, and nutritional value of conventional meat [9,10].The maturation of a bioartificial muscle (BAM) necessitates supportive structures that function to promote tissue formation, providing mechanical stability and cell-attachment sites that prolong the survival of myoblasts and myotubes, thereby ensuring extended organoid survival [11].
Traditionally, animal-derived proteinaceous hydrogel systems, such as collagen and fibrin, have been extensively used for muscle tissue engineering and were investigated for their applicability to the development of potential treatments and drug screening methodologies [12].As extracellular matrix (ECM) proteins, these hydrogels present cell attachment sites and fibrous constituents, aiding cells in adherence, spreading, and migration.Such systems rely on compaction to enable cell-cell contact (which is imperative for myogenic fusion into myotubes) and depend on anchorage to induce tension, which results in cell alignment, priming the construct for differentiation.The development of a uniform tissue in which cells are aligned via tension and guidance by fibrous structures, thereby promoting sustained myotube attachment, is an indispensable aspect of tissue maturation [13].However, these systems are animal-based and hence cannot be applicable to animal component-free product development.While diverse options for plant-based polysaccharides and decellularized materials have been explored to support BAM formation [5,14], their reduced degradability, inadequacy in creating tension, absence of mechanical support, and lack of attachment cues for myocytes hamper BAM viability.
Alginate is a commonly employed polysaccharide for muscle tissue engineering because its tunable mechanical and physical properties are well tailored to cellular requirements, alongside well-established options for peptide functionalization [15].The presence of calcium (an ionic cross-linker) significantly influences the tissue formation and gel-contraction behavior of alginate hydrogels.The dynamic nature of this crosslinking facilitates tunable mechanical properties and degradation of the tissue, adapting to the evolving requirements of the satellite cells, as they spread, differentiate, and fuse into myotubes.Nevertheless, alginate-based systems lack fibrous components akin to those available in natural ECM and collagen-based hydrogels, which benefit tissue formation and stability [16,17].Various studies have attempted to address these limitations, often through the integration of a secondary component.
For the selection of a suitable secondary material for fiber formation, there were a number of considerations that needed to be taken into account.A careful evaluation of alternatives suggested zein, a heterogeneous inherently hydrophobic protein mixture isolated from maize (Zea mays) [18], as a possible candidate, also due to its wide use in the food industry as a non-allergenic proteinaceous component.Zein primarily consists of alpha-zein (a 19 kDa glutamine-rich protein, which is the predominant component of zein), which has been established as cytocompatible and is known to be amenable to electrospinning [19,20] due to its beneficial charge distribution compared to other interesting materials, such as soy protein isolate or gluten [18].Another important aspect is the hydrophobicity of zein, which makes it more stable in aqueous solution than other plant-based materials such as pullulan, soy protein, or maltodextrin [18].Blending fibrous components has been shown to improve the mechanical properties of hydrogels, resulting in hybrid systems termed fiber-hydrogel composites (FHCs) [21].
Electrospinning provides an attractive method for producing fibers for hydrogel integration.Electrospun fibers are easy to fabricate, and the method is amenable to upscaling, while their fibrous structure can mimic natural ECM constituents, which, in combination with the aforementioned properties of the primary biomaterial, can assist tissue formation and maturation.Prior research has demonstrated convincing proof of this principle in animal-based and non-edible systems, for example, employing murine C2C12 cells encapsulated within gelatin-based hydrogels, with secondary fibrous compounds fabricated from polycaprolactone (PCL) [22].Translating these advantages into a cultivated meat system, however, necessitates an animal-free and food-compatible method.
In this study, we aimed to enhance the mechanical and physical attributes of an alginate hydrogel to improve cellular adhesion and compaction of 3D skeletal muscle tissues.We achieved this by incorporating electrospun zein fibers, leading to improved cell alignment and scaffold stability to support myogenic differentiation and maturation.

Electrospinning of Zein Fiber Solutions
In order to produce electrospun zein fibers, which can be processed into short stranded fibers (SSFs) and incorporated into RGD-functionalized alginate hydrogels (Figure 1), to improve tissue formation and cell alignment, we first optimized the electrospinning conditions.We characterized and compared five different solutions of 20, 25, 28, 30, and 35 wt% zein dissolved in a 1:1 mixture of acetic acid and ethanol (Table 1).We measured the physical properties of these solutions, including conductivity, surface tension and viscosity, which can affect the electrospinning process and fiber morphology.

Electrospinning of Zein Fiber Solutions
In order to produce electrospun zein fibers, which can be processed into short stranded fibers (SSFs) and incorporated into RGD-functionalized alginate hydrogels (Figure 1), to improve tissue formation and cell alignment, we first optimized the electrospinning conditions.We characterized and compared five different solutions of 20, 25, 28, 30, and 35 wt% zein dissolved in a 1:1 mixture of acetic acid and ethanol (Table 1).We measured the physical properties of these solutions, including conductivity, surface tension and viscosity, which can affect the electrospinning process and fiber morphology.The conductivity and viscosity of the different solutions correlated with the spinning results, which showed decreased viscosity and increased conductivity at lower zein concentrations, resulting in thin fiber and bead formation, which was undesirable for the short-stranded fibers we aimed to fabricate (Figure 2, Table 1).The opposite trend was seen as the zein concentration was increased to 28, 30, and 35 wt%, which resulted in thicker fibers.However, at concentrations higher than 30 wt%, the Taylor cone did not form during the electrospinning process, which led to inhomogeneous fiber morphologies (Figure 2, Table 1).Since 28 wt% zein proved most amenable to a robust electrospinning process and yielded the most promising fibrous zein sheets with homogeneous fiber size distribution, we proceeded with this solution for subsequent experiments.The conductivity and viscosity of the different solutions correlated with the spinning results, which showed decreased viscosity and increased conductivity at lower zein concentrations, resulting in thin fiber and bead formation, which was undesirable for the short-stranded fibers we aimed to fabricate (Figure 2, Table 1).The opposite trend was seen as the zein concentration was increased to 28, 30, and 35 wt%, which resulted in thicker fibers.However, at concentrations higher than 30 wt%, the Taylor cone did not form during the electrospinning process, which led to inhomogeneous fiber morphologies (Figure 2, Table 1).Since 28 wt% zein proved most amenable to a robust electrospinning process and yielded the most promising fibrous zein sheets with homogeneous fiber size distribution, we proceeded with this solution for subsequent experiments.

Zein Fibers Can Be Processed into Cytocompatible Short Stranded Fibers
After manufacturing electrospun zein fibers, we investigated the cytocompatibility of the fibrous zein sheets in a serum-free cell culture system, using primary bovine satellite cells (SCs).Promisingly, we observed that cells were able to attach and spread on the zein structures within 24 h without additional peptide functionalization (Figure 3A,B).This

Zein Fibers Can Be Processed into Cytocompatible Short Stranded Fibers
After manufacturing electrospun zein fibers, we investigated the cytocompatibility of the fibrous zein sheets in a serum-free cell culture system, using primary bovine satellite cells (SCs).Promisingly, we observed that cells were able to attach and spread on the zein structures within 24 h without additional peptide functionalization (Figure 3A,B).This observation suggests that zein protein as a secondary compound adds additional attachment sites to the 3D alginate construct and thus could improve cell-gel interaction.In order to form FHCs in which the dynamicity of the hydrogel is maintained, further processing of the zein sheets into SSFs was required.We first tested various electrospinning parameters to optimize the alignment of fiber scaffolds and found that increasing the rotation rate of the collector from 200 to 2500 rpm substantially improved fiber alignment.Both the non-aligned and aligned fibers were processed into SSFs using ultrasonication.We observed that processing of aligned zein scaffolds resulted in the reduced clustering of SSFs compared to the non-aligned fibers (Figure 3C,D).

Zein Fiber Addition Leads to Faster Biomaterial Degradation
To investigate the effect of zein fibers on the mechanical and physical properties of an alginate hydrogel and to understand the interactions between alginate polymers and zein fibers, we blended the SSFs at two different concentrations (0.1 and 0.5 wt%) and

Zein Fiber Addition Leads to Faster Biomaterial Degradation
To investigate the effect of zein fibers on the mechanical and physical properties of an alginate hydrogel and to understand the interactions between alginate polymers and zein fibers, we blended the SSFs at two different concentrations (0.1 and 0.5 wt%) and investigated the gel response in terms of stiffness, relative remaining mass, and swelling behavior (Figure 4A-C), since these properties facilitate cell migration, morphology and indirectly affect differentiation capacity.Alginate stiffness upon calcium crosslinking did not differ significantly; however, a trend of decreasing stiffness with increasing fiber concentration was observed (Figure 4A).Correlating with this result, we saw enhanced degradation of the gel with increasing fiber addition (Figure 4C).These two results in combination show that the fiber addition affects the mechanical properties that the cells sense when they are encapsulated during BAM formation.Additionally, we observed that the swelling behavior of the gel was affected by fiber addition (Figure 4B), which could be linked to the hydrophobicity of zein.

Addition of Zein Fibers Improves Compaction during Cultured Muscle Formation
After the addition of zein fibers to RGD-functionalized alginate (Figure S1), FHCs were tested in a 3D tissue culture system.The first step for tissue formation in a self-assembling hydrogel is cell-driven compaction [23].The majority of observed compaction occurred between days 0 and 3, when we also observed the most significant differences between the three groups (Figure 5A,B).While the final extent of compaction was not affected by the addition of zein fibers, the rate of BAMs compaction was substantially Alginate stiffness upon calcium crosslinking did not differ significantly; however, a trend of decreasing stiffness with increasing fiber concentration was observed (Figure 4A).Correlating with this result, we saw enhanced degradation of the gel with increasing fiber addition (Figure 4C).These two results in combination show that the fiber addition affects the mechanical properties that the cells sense when they are encapsulated during BAM formation.Additionally, we observed that the swelling behavior of the gel was affected by fiber addition (Figure 4B), which could be linked to the hydrophobicity of zein.

Addition of Zein Fibers Improves Compaction during Cultured Muscle Formation
After the addition of zein fibers to RGD-functionalized alginate (Figure S1), FHCs were tested in a 3D tissue culture system.The first step for tissue formation in a self-assembling hydrogel is cell-driven compaction [23].The majority of observed compaction occurred between days 0 and 3, when we also observed the most significant differences between the three groups (Figure 5A,B).While the final extent of compaction was not affected by the addition of zein fibers, the rate of BAMs compaction was substantially increased.On day 1, BAMs incorporating 0.1 and 0.5 wt% zein-SSFs showed significantly increased compaction compared to the control group (Figure 5A,B).To investigate the structure and distribution of zein-SSFs within the BAM construct and the interaction of cells with the incorporated SSFs in more detail, we coupled the zein with a green fluorescent dye.After fixing 3D muscle tissues on days 3, 7 and 10, we could visualize spreading and alignment of the cells via F-actin staining, which was enhanced with the addition of 0.1 wt% zein (Figure 5C).The addition of 0.5 wt% zein-SSFs, on the other hand, showed decreased F-actin expression and reduced cell alignment.The incorporated SSFs did not maintain their fibrous structure throughout the culture period but instead started to cluster into spherical structures, which subsequently degraded over time (Figure 5c).

Zein Fiber Addition Improves Protein Yield and Metabolic Activity
Having examined morphological changes during the course of BAM cultures, we next looked into cellular metabolic activity, including the accumulation of protein, in order to assess the extent of myogenic differentiation.Total protein measurements showed protein accumulation in both the control and 0.1 wt% zein, while the 0.5 wt% zein group showed the highest total protein yield on day 3, which did not accumulate further on days 7 and 10.The 0.1 wt% zein group showed increased protein accumulation on days 7 and day 10 compared to the control group (Figure 6A).To investigate the structure and distribution of zein-SSFs within the BAM construct and the interaction of cells with the incorporated SSFs in more detail, we coupled the zein with a green fluorescent dye.After fixing 3D muscle tissues on days 3, 7 and 10, we could visualize spreading and alignment of the cells via F-actin staining, which was enhanced with the addition of 0.1 wt% zein (Figure 5C).The addition of 0.5 wt% zein-SSFs, on the other hand, showed decreased F-actin expression and reduced cell alignment.The incorporated SSFs did not maintain their fibrous structure throughout the culture period but instead started to cluster into spherical structures, which subsequently degraded over time (Figure 5c).

Zein Fiber Addition Improves Protein Yield and Metabolic Activity
Having examined morphological changes during the course of BAM cultures, we next looked into cellular metabolic activity, including the accumulation of protein, in order to assess the extent of myogenic differentiation.Total protein measurements showed protein accumulation in both the control and 0.1 wt% zein, while the 0.5 wt% zein group showed the highest total protein yield on day 3, which did not accumulate further on days 7 and 10.The 0.1 wt% zein group showed increased protein accumulation on days 7 and day 10 compared to the control group (Figure 6A).To quantitatively compare the changes in muscle differentiation through the addition of zein fibers, a selection of muscle-specific proteins was measured.Desmin was chosen as a marker for early fusion, while the myosin heavy chain showed progression in the differentiation (often referred to as maturation).The group with 0.1 wt% zein-SSFs showed an earlier increase in both desmin and the myosin heavy chain compared with the control group (Figure 6B,C).The group with 0.5 wt% zein fibers showed significantly reduced expression of muscle proteins, which also correlated with the reduced actin fibers and alignment previously observed (Figures 4C and 6B,C).Other muscle-specific proteins such as alpha-actin-1, alpha-actinin, and myoglobin were measured using Western blot analysis and showed similar trends to the ELISAs (Figure 6D).To quantitatively compare the changes in muscle differentiation through the addition of zein fibers, a selection of muscle-specific proteins was measured.Desmin was chosen as a marker for early fusion, while the myosin heavy chain showed progression in the differentiation (often referred to as maturation).The group with 0.1 wt% zein-SSFs showed an earlier increase in both desmin and the myosin heavy chain compared with the control group (Figure 6B,C).The group with 0.5 wt% zein fibers showed significantly reduced expression of muscle proteins, which also correlated with the reduced actin fibers and alignment previously observed (Figures 4C and 6B,C).Other muscle-specific proteins such as alpha-actin-1, alpha-actinin, and myoglobin were measured using Western blot analysis and showed similar trends to the ELISAs (Figure 6D).
To further examine the metabolic activity of the myoblasts, glucose and glutamax consumption were measured, as well as the respective accumulation of lactate and ammonia (Figure 6E-H).Overall, the metabolic activity of the cells was increased via the addition of zein-SSFs, suggesting that the construct viability was increased, leading to longer-lasting tissues (Figure 6E-H).Contrary to the glucose, glutamax and lactate results, ammonia accumulation was reduced in the 0.1 wt% zein fiber group (Figure 6G).

Discussion
The primary objective of this study was to facilitate the assembly of skeletal muscle tissue in an alginate hydrogel system by improving the compaction and structural stability.For the creation of engineered muscle tissue, it is crucial to establish a balance between hydrogel stability and controlled degradation.The former contributes to early tissue formation, while the latter enables cell spreading and compaction [24].The accelerated degradation of the hydrogel, as a result of short-stranded zein fiber addition, aims to allow cells to align, facilitating the building up of tension through the mechanical function of the formed tissue as a prerequisite to myoblast fusion and myocyte maturation [25].Our approach involved the development of fiber hydrogel composites (FHCs) through the incorporation of short-stranded zein fibers into alginate hydrogels, with the aim of mimicking the stiffness and structural features of native ECM and extensively studied animal-derived hydrogels.
As a first step to making alginate FHCs, we fabricated and fragmented electrospun fibrous zein scaffolds based on previously described methods [19,20,22,26].The successful formation of a stable Taylor cone (also known as an 'electrohydrodynamic jet') was contingent upon the optimization of parameters such as the viscosity, conductivity and surface tension of the spinning solution, in combination with the applied voltage [27].The electrospinning of zein, due to its hydrophobic properties, commonly employs acetic acid and organic solvents, and the choice of solvent is known to influence the electrospinning process through the different degrees of protein unfolding they induce [28,29].To illustrate this, Selling et al. have shown that zein fibers electrospun from alcoholic solutions adopt a ribbon-like morphology, while fibers electrospun with acetic acid solutions resulted in more rounded fiber morphologies at similar concentrations [29].This can be explained by the lower vapor pressure of acetic acid, which reduces the evaporation at the needle tip and thus allows for more robust round fiber formation [29,30].In the present study, we optimized the spinning with a mixture of both acetic acid and ethanol.Spinning solutions with 20 and 25 wt% zein failed to form Taylor cones and thus led to heterogenous fiber formation due to their low viscosity and consequently low degree of polymer entanglement [29].While increased viscosity and reduced conductivity stabilized Taylor cone formation, 30 and 35 wt% zein solutions caused needle clogging.However, homogenous fibers of approximately 600 nm diameter could be achieved with 28 wt% zein solution.
Following ultrasonication, zein fibers were homogeneously incorporated into alginate hydrogels by blending two different final concentrations (0.1 and 0.5 wt%).After zein fiber addition, we observed disparities in swelling and degradation behaviors.Immediately after gel formation, swelling was significantly reduced, which can be interpreted as a function that is introduced by the hydrophobicity of the zein fibers.Mao et al. similarly observed that mixing hydrophobic and fragmented PCL fibers into alginate/gelatin hydrogels resulted in a reduced swelling behavior compared to hydrogels alone [22].While showing trends towards reduced stiffness with increasing fiber concentration, no significant differences could be observed between groups.Degradation was enhanced upon increasing zein fiber concentration, suggesting that the addition of the secondary component interfered with the intermolecular interactions between alginate polymer chains involving divalent calcium ions (Figure S2).Since zein is rich in hydrophobic amino acids, such as glutamine, proline, alanine and leucine, it is less abundant in anionic carboxylate residues [18].These carboxylate residues are involved in ionic crosslinking with divalent ions, leading to improved gelation.Previous work has shown that the alkaline hydrolysis of silk fibers creates anionic carboxylate residues, which improves the mechanical properties upon mixing of a small fraction with alginate [31], indicating that these carboxylate residues are imperative for ionic crosslinking and improved gelation.Another way to improve the interaction of SSFs with the alginate network could be to electrospin alginate together with zein to allow SSFs to participate in ionic crosslinking.
The enhanced degradation concurs with differences we observed in early tissue assembly, timing and extent of compaction behavior, and actin fiber formation.The compaction of BAMs usually occurs within the first 72 h after cell encapsulation and is based on both alginate degradation dynamics and cell-driven tissue reorganization as cells interact with the biomaterial blend.Within the initial 72 h timeframe, BAMs displayed an enhanced compaction rate and increased degradation due to zein-SSF presence.The consequent increase in tension, similar to collagen-based systems, led to improved actin fiber assembly and alignment.Notably, cell alignment and tension have previously been linked to enhanced myogenic differentiation [32][33][34].Yeo et al. demonstrated this by showing a higher degree of myotube alignment and myogenic differentiation on aligned PCL/alginate scaffolds compared to non-aligned scaffolds [33].Similarly we observed that the presence of 0.1 wt% zein-SSF improved actin protein expression, accompanied by a tension buildup around the stainless steel pillar, leading to improved early-stage differentiation.
It is desirable for the main protein fraction of a cultivated meat product to be cellderived in order to achieve meat mimicry, but, ultimately, a balance must be struck between structural stability for cell guidance and a minimum quantity of plant-based material in the final product.The improvements in tissue formation and alignment lead to more stable and durable constructs needed for maturation and thus protein accumulation, which is important for the quality and cost efficiency of the final product.As previously mentioned, texture and nutritional value are achieved though the sufficient maturation of the muscle fibers.Furthermore, taste, cooking behavior and water retention are key factors that determine cultivated meat quality.For the cooking behavior and final taste, the Maillard reaction plays a key role and can be further enhanced by resident zein fibers.Furthermore, the hydrophobicity of zein could play an important role in the water-holding capacity of the cultivated meat product.

Conclusions
In the present work, we show that the addition of electrospun short-stranded zein fibers facilitated hydrogel degradation, resulting in faster compaction, better cell-gel interaction and enhanced alignment of bovine muscle precursor cells.We conclude that edible short-fiber-hydrogel composites are a promising approach to support the optimal formation of 3D constructs by improving tissue stability and thus prolonging culture duration.This work paves the way for creating animal-free and environmentally favorable tissue-engineering approaches for a cultivated meat product.

Viscosity Measurements
Dynamic viscosity (mPa.s) of zein solutions at 25 • C was determined with a rotational viscometer (ViscoQC 300, Anton Paar GmbH, Graz, Austria) equipped with a concentric cylinder measuring system (CC26).Measuring volume was 10 mL with a minimum torque of 10%.A constant rotational speed was used to determine the dynamic viscosity value with 20, 10 and 5 rpm used for the 20-28, 30 and 35% zein solutions, respectively.

Conductivity Measurements
Conductivity (µS cm −1 ) of zein solutions at room temperature was determined with a SevenCompact pH/Ion meter (S220, Mettler Toledo, Columbus, OH, USA) equipped with a conductivity probe.

Electrospinning
Zein solutions were charged to 25 kV with a high-voltage power supply (IME).Solutions were spun at a flow rate of 2 mL h −1, and fibers were collected on a grounded rotating stainless steel cylinder (diameter, 90 mm) with a distance of 90 mm between needle and collector (Figure S3).Experiments were carried out at 25 • C and 40% relative humidity.

Scanning Electron Microscopy
Fiber morphology was analyzed using a scanning electron microscope (JSM-6010LV Plus, Jeol, Tokyo, Japan).Fibers were sputtered with gold prior to imaging (JFC-1300 10BA, Jeol).Average fiber diameters were measured using ImageJ, taking an average of 100 fibers for each sample.

Fluorescently Labeled Zein
Zein was fluorescently labeled by reacting its lysine residues with the fluorescent dye derivative Atto 488 NHS ester (ATTO-TEC, AD 488-31).Zein was dissolved in ethanol at 10 wt%, and 50 mM Atto 488 NHS ester was added and stirred overnight in the dark.Fluorescently labeled zein fibers were created by mixing zein solution (Section 4.1.1)with the fluorescently labeled zein solution at 1:100 dilution and electrospinning, as previously described (Section 4.1.4).

Synthesis of RGD-Functionalized Alginate
Sodium alginate (L3; KIMICA) was purified via dialysis (3.5-kDa membrane) at a 1 wt% concentration in water for 3 days at room temperature.The water was replaced daily, and the solution was lyophilized (L-200, Buchi, Flawil, Switzerland) to obtain the solid material.Next, purified alginate was dissolved in 100 mM MES and 300 mM NaCl buffer at pH 6.5 to create a 1 wt% solution.Once dissolved, N-hydroxysulfosuccinimide sodium salt (sulfo-NHS; TCI) and 1-Ethyl-3-(3-dimethylaminopropyl) carbodiimide hydrochloride (EDC-HCl; Sigma-aldrich) were added at a concentration of 0.47 and 0.95 mg mL −1 , respectively.After 30 min, the pH was adjusted to 8.0, and NH 2 -G4RGDSP-COOH (Biomatik, Kitchener, ON, Canada) was added at a concentration of 1 µg mL −1 and allowed to react for 20 h.The reaction mixture was purified in 100, 50, 25 and then 0 mM NaCl for 3 days, replaced daily and finally lyophilized to obtain the RGD-functionalized alginate product.
The product was dissolved in D 2 O and transferred to an NMR tube.One-dimensional 1 H spectra were recorded on a Bruker Ascend™ 700 MHz NMR spectrometer at 299.7 K.

Gel Degradation Assays
Purified and lyophilized alginate prepared at a concentration of 0.9 wt% in PBS (Gibco; #10010023, Waltham, MA, USA) was mixed with short-stranded zein fibers at concentrations of 0.1 wt% and 0.5 wt% and crosslinked in 100 mM CaCl 2 for 5 min.Crosslinked hydrogels were washed once with basal media and incubated in PBS at 37 • C for a maximum of 72 h.Samples were taken at 0, 24 and 72 h.After the removal of PBS, wet weight was measured, and post-lyophilization, dry mass was determined at the respective timepoints.

Mechanical Properties
Effective Young's moduli were determined using a PIUMA nanoindenter (Optics11, Amsterdam, The Netherlands) on crosslinked hydrogels.Hydrogels were crosslinked around stainless steel pillars as shown in Figure 4. Gels were maintained in a buffer containing 50 mM CaCl 2 , 50 mM 3-(N-morpholino)propanesulfonic acid and 150 mM NaCl.Indentations were performed using a probe with a tip radius of 51 µm and cantilever stiffness of 0.43 N m −1 .Effective Young's modulus was determined by fitting a Hertzian Contact model over 80% of the load-indentation curve.4.2.5.3D Cell Culture RGD-functionalized alginate was dissolved at a concentration of 1.8 wt% in PBS and mixed with short-stranded zein fibers (0, 0.1 and 0.5 wt%).Bovine SCs were expanded in SFGM (Supplementary Table S1) and, after harvesting, resuspended at 1.2 × 10 7 cells mL −1 in serum-free differentiation medium (SFDM Supplementary Table S1).Cell suspension and alginate/zein solutions were mixed at a 1:1 ratio.Gel mixtures were injected around stainless steel pillars and crosslinked using immersion in 100 mM CaCl 2 for 5 min.After crosslinking, BAMs were washed and incubated in SFDM.Medium was changed on days 3 and 7, and from day 3 onwards, SFDM was additionally supplemented with 10 µM acetylcholine.After a total of 10 days, BAMs were harvested for protein quantification and confocal microscopy.For compaction assays, BAMs were imaged every day during the 7-day period (DC-TZ90, Panasonic Lumix, Kadoma, Japan).Images were analyzed in ImageJ.

ELISAs
Protein extracts were tested for relative desmin and slow myosin heavy chain (MYH7) content using in-house ELISAs.For desmin ELISA, samples were diluted to 20 µg mL −1 total protein in carbonate coating buffer (pH 9.5) supplemented with 5% RIPA and 100 µg mL −1 bovine serum albumin (BSA), and a Nunc Maxisorp plate was added (Invitrogen, Waltham, MA, USA, 44-2404-21).After a 2 h incubation period, wells were washed and blocked with 10 mg mL −1 BSA in TBS.Samples were stained with indicated primary and respective secondary antibodies (Supplementary Table S2).For myosin ELISAs, plates were incubated overnight with a capture antibody (Supplementary Table S2) in TBS at 4 • C.After blocking, samples diluted to 100 µg mL −1 protein in TBS containing 0.1% Tween-20 and 100 µg mL −1 BSA were added to the pre-coated and pre-blocked ELISA plates.Following 2 h of incubation, biotinylated detection antibody was added (biotinylation of carrier and preservation-free antibody was performed with the Abcam Lightning Link biotinylation kit, ab201795), and the respective secondary antibody was added (Supplementary Table S2).After a final wash, signals of both ELISAs were visualized using 1-step Ultra TMB ELISA

Figure 3 .
Figure 3. Cell attachment and processing of electrospun fibers.(A) Scanning electron microscope (SEM) images showing cell attachment to zein fibers.Scale bar, 10 µm.(B) Fluorescence microscopy images of satellite cells attaching to zein fibers.Phalloidin, white; Hoechst, blue.Scale bar, 100 µm.(C) SEM images showing the morphology of aligned and non-aligned zein fibers before processing.Scale bar, 50 µm.(D) Brightfield microscopy images of zein fibers shown in C, post-processing with ultrasonication.Scale bars, 75 µm.

Figure 3 .
Figure 3. Cell attachment and processing of electrospun fibers.(A) Scanning electron microscope (SEM) images showing cell attachment to zein fibers.Scale bar, 10 µm.(B) Fluorescence microscopy images of satellite cells attaching to zein fibers.Phalloidin, white; Hoechst, blue.Scale bar, 100 µm.(C) SEM images showing the morphology of aligned and non-aligned zein fibers before processing.Scale bar, 50 µm.(D) Brightfield microscopy images of zein fibers shown in C, post-processing with ultrasonication.Scale bars, 75 µm.

Figure 6 .
Figure 6.Protein yield and metabolic changes after zein fiber addition.(A) Total protein measurements for BAMs with 0, 0.1 and 0.5 wt% zein fibers at indicated timepoints.Error bars indicate s.d., n = 2.No statistically significant differences were observed, with P-values > 0.05.(B) Desmin ELISAs in BAMs with 0, 0.1 and 0.5 wt% zein fibers.Error bars indicate s.d., n = 2. p-values > 0.05.(C) Same as B, but slow myosin heavy-chain ELISAs.Error bars indicate s.d., n = 2. P-values > 0.05.(D) Western blot of selected muscle-related proteins during myogenic differentiation, analyzed at indicated timepoints.(E) Lactate concentrations recorded in the culture medium at indicated timepoints.Values are normalized to day 0. p-values > 0.05.(F) As E, but for glucose concentrations.(G) As E, but for ammonia concentrations.(H) As E, but for glutamax concentrations.

Figure 6 .
Figure 6.Protein yield and metabolic changes after zein fiber addition.(A) Total protein measurements for BAMs with 0, 0.1 and 0.5 wt% zein fibers at indicated timepoints.Error bars indicate s.d., n = 2.No statistically significant differences were observed, with P-values > 0.05.(B) Desmin ELISAs in BAMs with 0, 0.1 and 0.5 wt% zein fibers.Error bars indicate s.d., n = 2. p-values > 0.05.(C) Same as B, but slow myosin heavy-chain ELISAs.Error bars indicate s.d., n = 2. P-values > 0.05.(D) Western blot of selected muscle-related proteins during myogenic differentiation, analyzed at indicated timepoints.(E) Lactate concentrations recorded in the culture medium at indicated timepoints.Values are normalized to day 0. p-values > 0.05.(F) As E, but for glucose concentrations.(G) As E, but for ammonia concentrations.(H) As E, but for glutamax concentrations.

Table 1 .
Characterization of zein solutions for electrospinning.

Table 1 .
Characterization of zein solutions for electrospinning.