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Cellobiose

Cellobiose is a consisting of two β-D-glucose molecules joined by a β(1→4) , making it the fundamental repeating unit of . It is classified as a due to its free anomeric carbon on one glucose unit, which allows it to participate in reactions. Chemically known as 4-O-β-D-glucopyranosyl-D-glucose, cellobiose has the molecular formula C₁₂H₂₂O₁₁ and a molecular weight of 342.30 g/mol. Cellobiose appears as a white solid and is produced primarily through the partial of , a major component of cell walls; it does not occur freely in nature but can be detected as an intermediate in organisms that metabolize material, such as certain and fungi. Biologically, cellobiose plays a key role in the degradation of , where it is an intermediate hydrolyzed to glucose. It acts as a substrate for enzymes such as cellobiose phosphorylase and , facilitating phosphorolytic pathways with energetic advantages in and aiding in the of compounds like (in engineered yeasts) or H₂O₂ for purposes. In human health contexts, cellobiose is used in diagnostic tests, such as the cellobiose/ permeability test, for conditions like and syndromes, as its absorption reflects intestinal function. Industrially, cellobiose is utilized as a in for production via enzymatic of , where overcoming cellobiose inhibition of cellulases is a key challenge. It has also received a GRAS notice from the FDA for use as a substitute for or in powdered formulas for young children (ages 1–3 years), as of 2024.

History and Discovery

Discovery and Isolation

The discovery of cellobiose emerged from foundational studies on , a major component of plant cell walls first isolated in pure form by French chemist Anselme Payen in 1838. Payen extracted this insoluble from woody tissues using a combination of and treatments, recognizing it as a distinct chemical entity resistant to typical solvent extractions and naming it "cellulose" from the Latin for "living cell." This isolation laid the groundwork for later efforts to elucidate cellulose's structure through degradative methods, though cellobiose itself remained unidentified for decades. The first preparation of cellobiose occurred in 1879 when Dutch chemist Augustinus Petrus Franchimont performed acetolysis on derived from , yielding cellobiose octaacetate as a crystalline product. Acetolysis, involving treatment with and , partially broke down the cellulose polymer into smaller fragments, allowing isolation of this acetylated derivative through recrystallization from solvents like or . Franchimont's work marked the initial recognition of a repeatable product from cellulose, though its exact nature was not fully characterized at the time. Confirmation of cellobiose as a came in 1901 through the efforts of Austrian chemists Zdenko Hans Skraup and Joseph König, who deacetylated Franchimont's octaacetate and analyzed the resulting compound, determining it consisted of two glucose units. They achieved this via mild acid followed by purification and characterization using and tests, establishing cellobiose's identity distinct from glucose or other monosaccharides. Subsequent isolations in the early , such as those by Karl Freudenberg in 1921, refined the process by optimizing acetolysis conditions to achieve yields up to 40%, often starting from purified linters or wood . Enzymatic approaches also emerged, employing crude preparations from fungi or to perform controlled , with products purified via fractional from aqueous . The isolation of cellobiose held profound historical significance, providing empirical evidence that cellulose is a linear of anhydroglucose units connected via β-1,4 linkages, as later confirmed through structural studies in the . This breakthrough shifted carbohydrate chemistry from empirical observations to a polymer-based understanding, influencing advancements in biochemistry and by revealing the repetitive motif in natural .

Nomenclature and Etymology

The name "cellobiose" is derived from "," reflecting its origin as a product of that , combined with the prefix "-bi-" to indicate its nature and the suffix "-ose" denoting a , following conventions established in carbohydrate chemistry. This etymological construction was first recorded in English between 1900 and 1905, coinciding with advances in isolating and characterizing plant-derived sugars. The systematic International Union of Pure and Applied Chemistry (IUPAC) name for cellobiose is 4-O-β-D-glucopyranosyl-D-glucose, which specifies the β- between two D-glucose units at the 4-position of the second glucose. An alternative nomenclature, β-D-glucopyranosyl-(1→4)-D-glucose, emphasizes the (1→4) connecting the anomeric carbon of the first glucose to the 4-position of the second, distinguishing cellobiose from , which features an α(1→4) linkage between identical glucose monomers. The evolution of cellobiose's nomenclature mirrors broader early 20th-century developments in science, where disaccharides like cellobiose were increasingly recognized as fundamental repeating units in such as , building on Emil Fischer's foundational work in the late on sugar configurations and linkages. Formal rules for naming linkages in disaccharides, as codified in IUPAC recommendations, emerged from collaborative efforts in the 1940s and 1950s, standardizing trivial names like cellobiose alongside systematic descriptors to facilitate structural comparisons across saccharides.

Chemical Structure

Molecular Composition

Cellobiose has the molecular formula \ce{C12H22O11}. It consists of two D-glucose monomers, each with the formula \ce{C6H12O6}, joined through a that removes one of (\ce{H2O}), yielding a total of 12 carbon atoms, 22 hydrogen atoms, and 11 oxygen atoms. The features eight hydroxyl (-\ce{OH}) groups, one glycosidic ether linkage connecting the two glucose units, and one at the reducing end. At the reducing end, cellobiose can exist in \alpha or \beta anomeric forms due to the hemiacetal, though the \beta-anomer predominates in solid state and natural occurrences. Cellobiose represents the disaccharide repeating unit within the cellulose polymer, which forms linear chains in plant cell walls.

Glycosidic Linkage and Conformation

Cellobiose features a β(1→4) glycosidic linkage, in which the anomeric carbon (C1) of one D-glucose unit forms an ether bond with the hydroxyl group at C4 of the adjacent D-glucose unit, resulting in the systematic name 4-O-β-D-glucopyranosyl-D-glucose. This β configuration inverts the anomeric orientation relative to maltose, which shares the same 1→4 linkage but with an α anomer, leading to distinct steric arrangements and polymer properties. The enables a predominantly extended, linear conformation of the , facilitating the formation of long chains in like . In this arrangement, both glucose units adopt conformations of their rings, with the β linkage promoting anti-periplanar orientation of the glycosidic torsion angles (φ and ψ), which minimizes steric hindrance and allows for intermolecular hydrogen bonding between the hydroxyl groups of adjacent units. These hydrogen bonds, particularly involving the ring oxygen and hydroxyls at and , contribute to the structural rigidity and stability observed in cellulose microfibrils. In projections, the β-anomer at the non-reducing end is represented with the glycosidic oxygen below the plane of the ring, highlighting the equatorial orientation of the linkage in the chair form. Unlike non-reducing disaccharides such as , which features an α(1→2) linkage between glucose and that locks both anomeric carbons, cellobiose retains a free anomeric hydroxyl at the reducing end, conferring properties due to the ability to open into an aldehyde form. Spectroscopic techniques have confirmed the β(1→4) linkage and conformational preferences. ¹H NMR studies in reveal chemical shifts consistent with the β , including downfield signals for H1 of the reducing end (around 4.6–5.2 ppm depending on ). NOE enhancements support a folded or extended population with specific torsion angles. ¹³C NMR data further validate the chair rings, with C1 resonances at approximately 100–105 ppm for the β-linked and C4 shifts indicating the glycosidic attachment. analyses of cellobiose crystals and analogs show lattice parameters aligning with the linear β(1→4) chain, with bond lengths of about 1.4 for the glycosidic oxygen-carbon and intermolecular distances of 2.7–2.9 .

Physical Properties

Appearance and Solubility

Cellobiose is a , odorless, crystalline solid at . This appearance is characteristic of its high-purity forms, which are typically supplied as fine powders for and use. Due to its hygroscopic nature, cellobiose readily absorbs moisture from the atmosphere, leading to the formation of hydrates that can affect its handling and storage. Proper storage in dry conditions is essential to prevent clumping or from humidity exposure. In terms of , cellobiose shows moderate solubility, with approximately 12 g dissolving in 100 mL of at 20°C. It is insoluble in , and remains insoluble in nonpolar solvents such as and . This solubility profile reflects its polar structure, favoring aqueous environments over organic ones. Cellobiose possesses a mildly sweet , consistent with its composition. It is generally recognized as non-toxic for consumption in moderate amounts, though high doses exceeding 20 g in a single intake or 15 g twice daily may cause gastrointestinal discomfort such as or . Regulatory assessments confirm its safety as a ingredient at proposed intake levels below 290 mg/kg body weight per day. Commercial cellobiose is available in high-purity grades, often exceeding 98% as determined by HPLC analysis, with residual impurities primarily stemming from incomplete of during production. These impurities, such as glucose monomers, are minimized in pharmaceutical and biochemical applications to ensure consistency.

Thermal and Optical Properties

Cellobiose exhibits thermal stability in its crystalline form, though the solid remains intact until without a distinct at around 225–230°C, often releasing or fragmenting into simpler sugars like glucose under heating conditions. The density of crystalline cellobiose is reported in the range of 1.27–1.61 g/cm³ at ambient temperatures, reflecting its compact molecular packing in the solid state. Optically, cellobiose is chiral and displays a of [\alpha]_D^{20} +34^\circ (c = 10 in ) at equilibrium, a value achieved after equilibrates the α-anomer (initially higher rotation) to the more stable β-form over about 15 hours in solution. This optical activity arises from the centers in its glucose units linked by the β-1,4-glycosidic bond. For , aqueous solutions of cellobiose show values around 1.35, increasing slightly with concentration due to the solute's contribution to the medium's optical . Solid-state approximates 1.47–1.50, similar to related such as . These properties aid in spectroscopic identification and purity assessment of cellobiose samples.

Chemical Properties

Reactivity as a Reducing Sugar

Cellobiose functions as a owing to the presence of a free group at the anomeric carbon (C1) of its reducing glucose unit, which can tautomerize to an form in . This group enables cellobiose to reduce alkaline (II) solutions, such as those in Benedict's or Fehling's , leading to the formation of a brick-red precipitate of cuprous oxide (Cu₂O). The confirms the reducing capability, with the intensity of the color change proportional to the concentration of the reducing end. Under acidic conditions, cellobiose undergoes via cleavage of its β-1,4-glycosidic bond, yielding two molecules of D-glucose. This process is catalyzed by protons that protonate the glycosidic oxygen, facilitating bond rupture and subsequent ring opening. The hydrolysis rate for cellobiose is notably slower than that of , primarily due to the β-configuration of the linkage, which imparts greater resistance through increased steric hindrance and altered electronic stabilization compared to the α-1,4 bond in ; activation energies for cellobiose hydrolysis are reported around 30-32 kcal/mol, higher than the ~28 kcal/mol for . Oxidation of cellobiose with , which contains ammoniacal , targets the form at the reducing end, converting it to a and depositing a silver mirror on the reaction vessel. The product is cellobionic acid (4-O-β-D-glucopyranosyl-D-gluconic acid), where only the reducing glucose unit is oxidized while the non-reducing unit remains intact. This selective oxidation highlights the reactivity confined to the free anomeric center. In , cellobiose exhibits , interconverting between its α and β anomers at the reducing end through ring opening and reclosure, reaching an composition of approximately 38% α and 62% β, akin to free glucose. The process follows , with rate constants at 20°C ranging from 0.015 to 0.025 min⁻¹ depending on and concentration, slower than for monosaccharides due to the stabilizing influence of the glycosidic linkage. The pKₐ for ionization of the hydroxyl group is 12.39, reflecting its weak acidity and role in the mutarotational .

Derivatives and Modifications

Cellobiose octaacetate is a prominent derivative formed by the complete of all eight hydroxyl groups on the , resulting in the esterification with acetic acid residues. This compound, with the molecular formula C_{28}H_{38}O_{19}, is synthesized via acetolysis of using and as a catalyst, which cleaves the into the unit while simultaneously acetylating it. The process, first described by Franchimont and refined in subsequent studies, yields the α-anomer predominantly and enables isolation through recrystallization. The octaacetate exhibits enhanced solubility in organic solvents such as , acetone, and compared to unmodified cellobiose, facilitating its handling in settings. It has a of 225°C and is commonly employed for the purification of cellobiose derivatives and structural elucidation through techniques like and NMR spectroscopy. Deacetylation of cellobiose octaacetate, typically achieved with in , regenerates the parent cellobiose in high yield, providing a reversible modification route. Other notable derivatives include the octamethyl ether, prepared by exhaustive methylation of cellulose with dimethyl sulfate or methyl iodide, followed by acetolysis to isolate the crystalline octamethyl cellobiose. This ether derivative, with formula C_{20}H_{38}O_{11}, serves in studies of glycosidic bond stability and conformational analysis due to its increased lipophilicity. Phosphate esters of cellobiose, such as cellobiose-6'-phosphate, are chemically synthesized via phosphorylation of protected cellobiose intermediates using phosphoryl chloride or similar reagents, and are utilized in biochemical research to probe enzyme-substrate interactions in phosphorolytic pathways. These derivatives, particularly the octaacetate, aid in chromatographic separations for analytical purposes, allowing resolution of cellobiose from complex mixtures in structural studies.

Synthesis and Production

Natural Sources and

Cellobiose is primarily encountered as a transient intermediate during the partial of , the most abundant in walls, rather than as a directly synthesized . In natural settings, it arises from the action of endogenous enzymes or microbial cellulases that cleave β-1,4-glycosidic bonds in chains, releasing cellobiose as a soluble product before further breakdown to glucose. This process occurs during cellulose turnover in growing or senescing tissues, where cellobiose serves as a , signaling stress and enhancing responses. Trace amounts of free cellobiose are detectable in various plant-derived foods and materials, reflecting its role in natural degradation pathways. For instance, it is present in at concentrations of 0.06–0.28 g/100 g, as well as in developing grains, pine needles, corncobs, and fermented plant-based products such as juices. In , such as or agricultural residues, cellobiose typically constitutes less than 1% of the total content, underscoring its ephemeral nature. While some produce cellulose-like structures in their cell walls, cellobiose appears as a minor during their β-glucan breakdown, though specific concentrations remain low and context-dependent. Microbial systems contribute significantly to cellobiose formation in natural environments, particularly in and ruminant guts where lignocellulosic occurs. Fungi such as and certain bacteria employ cellobiohydrolases (e.g., cellobiohydrolase I) to processively hydrolyze from its non-reducing ends, yielding cellobiose as the primary product. This enzymatic release facilitates microbial carbon acquisition but also results in transient accumulation of cellobiose in culture media or digesta. In , analogous endo- and exoglucanases perform partial during hemicellulose remodeling, though cellobiose's role here is secondary to structural maintenance. Overall, cellobiose is not accumulated as a stable endpoint but is rapidly metabolized, limiting its steady-state levels in biological systems.

Laboratory and Industrial Synthesis

In laboratory settings, cellobiose is commonly produced through enzymatic hydrolysis of cellulose substrates, such as filter paper or microcrystalline cellulose, using cellulase enzyme complexes derived from fungi like Aspergillus niger. These complexes include endoglucanases and cellobiohydrolases that cleave β-1,4-glycosidic bonds to release cellobiose as the primary product, while β-glucosidase activity is minimized or removed—often via affinity precipitation with chitosan—to prevent further conversion to glucose and achieve higher selectivity. Yields typically range from 50% to 80% cellobiose in the soluble fraction, depending on enzyme loading, hydrolysis time (24–72 hours at 50°C), and process modifications like multistage filtration to reduce product inhibition. Acid hydrolysis is a historical laboratory method for isolating cellobiose from cellulose sources like cotton or wood pulp under mild acidic conditions to produce oligosaccharides including cellobiose, though it often requires separation from glucose and other products. Chemical synthesis of cellobiose in the laboratory traditionally employs the Koenigs-Knorr reaction, coupling a protected glucose derivative (e.g., acetobromoglucose) as the glycosyl donor with another glucose acceptor in the presence of silver salts or promoters to form the β-1,4-glycosidic linkage, followed by deprotection. This method, pioneered in early 20th-century work, suffers from low yields (often below 30%) due to stereoselectivity challenges and side reactions. Modern alternatives utilize enzymatic synthesis with glycosyltransferases or phosphorylases, such as cellobiose phosphorylase in a one-pot reaction from glucose-1-phosphate and glucose, achieving higher efficiencies (up to 80% yield) and enabling scalable preparation of isotopically labeled cellobiose for research. A recent advance (as of 2024) involves one-pot synthesis from sucrose using co-displayed sucrose phosphorylase and cellobiose phosphorylase in Pichia pastoris whole-cell biocatalysts, yielding up to 81 g/L cellobiose (81% theoretical yield) at 60°C in 24 hours, offering a sustainable alternative without cellulose substrates. On an industrial scale, cellobiose production leverages waste , such as agricultural residues or forest waste, through pretreatment (e.g., or dilute acid) to disrupt lignocellulosic structure, followed by enzymatic with commercial cocktails at high loadings (10–20% solids) and 45–50°C for 48–96 hours. This process generates cellobiose as a key intermediate, with overall yields exceeding 70% from fraction, though β-glucosidase supplementation is adjusted to retain cellobiose for downstream applications like biofuels. Scalability is enhanced by integrated approaches, recycling enzymes and achieving titers up to 20 g/L cellobiose from pretreated . Purification of cellobiose from hydrolysis mixtures typically involves ion-exchange chromatography using strong acidic cation-exchange resins (e.g., Na⁺ or Ca²⁺ forms) to separate it from glucose and other oligosaccharides, eluting with hot water (70°C) at a space velocity of 1.0 for ≥90% purity and 80% recovery. Final isolation is achieved by recrystallization from aqueous solutions (45–55% solids content), cooling to 20°C, and , yielding crystals of 93–98% purity with 40–70% recovery, suitable for commercial-grade product.

Biological Role

Role in Cellulose Degradation

Cellobiose serves as a key intermediate in the enzymatic degradation of , the primary structural component of cell walls. In this process, cellobiohydrolases (CBHs), such as CBH I and CBH II produced by fungi like , act on the crystalline regions of cellulose microfibrils. These exo-acting enzymes progressively cleave β-1,4-glycosidic bonds from the reducing or non-reducing ends of cellulose chains, releasing cellobiose disaccharides as the primary product. This end-wise is often the rate-limiting step in cellulose breakdown due to the recalcitrant nature of crystalline cellulose. Beyond its role as a degradation product, cellobiose functions as an inducer of in cellulolytic microorganisms. In fungi such as , cellobiose uptake via specific transporters activates signaling pathways that upregulate the transcription of genes encoding CBHs, endoglucanases, and β-glucosidases. This induction mechanism ensures that enzyme production is responsive to the presence of cellulosic substrates, optimizing resource allocation in nutrient-limited environments. However, excessive cellobiose accumulation can lead to feedback inhibition, where it competitively binds to CBHs and endoglucanases, slowing further and thereby regulating the overall rate to prevent enzyme overload. The hydrolysis of cellobiose to glucose is mediated by β-glucosidases, which complete the cellulose degradation pathway by cleaving the β-1,4-glycosidic bond in the disaccharide. These enzymes, often secreted extracellularly by microbes, alleviate product inhibition by converting cellobiose into utilizable glucose, facilitating efficient carbon assimilation. In natural ecosystems, this process is crucial for carbon cycling, as soil microbes and termite gut symbionts decompose plant-derived cellulose, recycling organic matter and releasing nutrients into the environment. For instance, in termite digestion, microbial consortia produce CBHs and β-glucosidases that generate and process cellobiose, contributing significantly to lignocellulose breakdown in tropical soils.

Metabolism in Organisms

In microorganisms, particularly cellulolytic such as those in the genera and Cellulomonas, cellobiose is primarily transported into the cell via ATP-binding cassette () permeases. Once internalized, cellobiose is metabolized through by β-glucosidases (cellobiases) to yield two molecules of glucose, which then enter for energy production, or via a phosphorolytic pathway catalyzed by cellobiose to produce glucose and glucose-1-phosphate, conserving ATP compared to the hydrolytic route. This dual-pathway utilization enhances efficiency in biomass-degrading microbes, enabling direct assimilation without extracellular accumulation of inhibitory cellobiose. In animals and humans, cellobiose exhibits poor absorption in the due to the absence of mucosal activity, leading to its by colonic rather than direct uptake. Consequently, ingested cellobiose remains largely indigestible in the upper gut and is utilized by gut , producing as metabolic byproducts. This property makes cellobiose a component in dual-sugar permeability tests, such as the cellobiose-mannitol assay, which assesses intestinal barrier function in disorders like celiac disease by measuring urinary excretion ratios. Plant metabolism of cellobiose plays a limited role, as it is primarily recognized as a minor in such as flowering s and , with no well-defined catabolic pathways. Cellobiose is generally non-toxic at low doses but can induce osmotic upon high ingestion (e.g., >20 g), as unabsorbed molecules draw into the intestinal lumen. As documented in metabolomic databases, cellobiose serves as an endogenous , underscoring its natural occurrence without adverse effects in those contexts. Evolutionarily, cellobiose metabolic machinery, including transporters and hydrolases, is conserved across diverse cellulolytic organisms from to fungi, facilitating efficient utilization in terrestrial ecosystems.

Applications and Uses

Medical and Diagnostic Applications

Cellobiose plays a key role in the oral cellobiose- test, a non-invasive method for evaluating to aid in diagnosing conditions like , celiac disease, and syndromes. This test measures the urinary excretion ratio of cellobiose to mannitol following oral ingestion, providing insight into the integrity of the intestinal barrier. Developed and validated in studies from the onward, it has demonstrated utility in detecting mucosal damage associated with these disorders. The standard protocol involves patients overnight before ingesting a solution containing 5 g of cellobiose and 2 g of , dissolved in 100 mL water. is then collected for 5 hours, and the cellobiose-to- ratio is determined using techniques like . In healthy individuals, the ratio is normally less than 0.025, reflecting intact paracellular pathways; elevated ratios (>0.025) signal increased permeability. The mechanism exploits cellobiose's larger molecular size (), which limits its to paracellular routes disrupted in disease states, while (a ) is readily absorbed transcellularly, serving as a control for overall efficiency. Clinical evidence supports the test's reliability for (IBD) and disease, with studies showing approximately 80-96% sensitivity for active and untreated cases, respectively, and fewer false positives compared to older screening methods like the D-xylose test. For instance, in cohorts of over 1,000 unselected patients, the test identified 96% of confirmed cases via jejunal correlation. It also aids in monitoring treatment response, such as gluten withdrawal in disease, where ratios normalize with barrier recovery. In , elevated ratios correlate with disease activity in the . The test is well-tolerated, with minimal side effects reported, primarily mild gastrointestinal upset like transient , and no serious adverse events in clinical trials. metabolism of cellobiose, involving to glucose by intestinal microbes, poses no additional risks in this context.

Industrial and Research Applications

Cellobiose serves as a key intermediate in the production of , where it is enzymatically hydrolyzed to glucose for subsequent into , playing a central role in second-generation biofuel processes that utilize . Engineered microorganisms, such as strains expressing cellobiose transporters and β-glucosidases, enable direct of cellobiose to , improving efficiency and reducing costs in consolidated bioprocessing approaches. In scientific research, cellobiose functions as a model compound for investigating hydrolases, including β-glucosidases and cellobiohydrolases, due to its structural similarity to chain ends. It is commonly employed in assays to measure kinetic parameters, such as inhibition by product accumulation, and to study -binding domains in cellulolytic s. For instance, real-time biosensors utilizing cellobiose dehydrogenase detect cellobiose release during , aiding in the optimization of biomass-degrading enzyme cocktails. Cellobiose exhibits mild sweetness, approximately 20% that of , positioning it as a potential low-calorie alternative in formulations. As a precursor, it is used in the enzymatic synthesis of cello-oligosaccharides, which serve as prebiotic components in nutraceuticals due to their non-digestible nature and ability to promote beneficial . Regulatory assessments have confirmed its safety for use as a ingredient in such applications. In industrial processes, cellobiose is commercially available from suppliers like , facilitating its incorporation into enzymatic treatments for and , where it supports assays for delignification efficiency by modeling products. Emerging research explores cellobiose in studies as an inducer of lignocellulolytic enzymes in fungi like , enhancing biomass conversion yields. Additionally, derivatives such as cellobiose sulfate, obtained from nanocrystals, are investigated in for surface modification of .

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