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NAD+

Endogenous metabolite / coenzyme

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1

capsule

1000mg

Lyophilized powder

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≥98%

NAD⁺ functions as a central electron carrier in redox biology and is indispensable for the maintenance of cellular energy metabolism, metabolic flux regulation, and enzymatic homeostasis across both cytosolic and mitochondrial compartments.

$120.00

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Form
Lyophilized
Molecular Formula
C21H27N7O14P2
Molecular Weight
663.43 g/mol
CAS Number
53-84-9
PubChem CID
5892
Research Data
NAD+ Level Decline
Intracellular NAD+ concentration vs. age (% of peak)
Literature
Cellular Ratio
Biological Intersections
Relative pathway engagement
Activity Profile
NAD+ Metabolic Profile
Mechanism
Cellular Pathway
01
SIRT1/SIRT3 Deacylase Activation
NAD+ accepts electrons from NADH in glycolysis, TCA cycle, and fatty acid oxidation, serving as essential electron carrier for ATP synthesis via OXPHOS.
02
PARP-1 DNA Repair and NAD+ Consumption Loop
NAD+ is consumed by sirtuins as co-substrate during protein deacylation. SIRT1/3 activation drives mitochondrial biogenesis, fatty acid oxidation, and stress resistance.
03
Mitochondrial Electron Transport (NADH/NAD+ Cycling)
PARP1/2 consume NAD+ during poly-ADP-ribosylation at DNA break sites, coordinating repair. Excessive DNA damage depletes NAD+ stores rapidly.
04
CD38 NADase Pathway
05
NAMPT Biosynthesis Axis
06
Anti-Inflammatory NF-κB Deacetylation
Metabolic Network
Biosynthesis Map
SIRT1/SIRT3 Deacylase Activation
NAD+ accepts electrons from NADH in glycolysis, TCA cycle,…
PARP-1 DNA Repair and NAD+ Consumption Loop
NAD+ is consumed by sirtuins as co-substrate during protein…
Mitochondrial Electron Transport (NADH/NAD+ Cycling)
PARP1/2 consume NAD+ during poly-ADP-ribosylation at DNA break sites,…
CD38 NADase Pathway
NAMPT Biosynthesis Axis
Anti-Inflammatory NF-κB Deacetylation
 NAD+ CENTRAL HUB
Sequence Analysis
Amino Acid Sequences
Single-letter residue map colored by physicochemical property class. Hover any residue for full name and position.
BPC-157
G E P P P G K P A D D A G L V
15Residues
-2Net Charge
1Basic
3Acidic
TB-500
L K K T E T Q
7Residues
+1Net Charge
2Basic
1Acidic
■ Hydrophobic ■ Polar ■ Positively Charged ■ Negatively Charged ■ Glycine
Research Focus
NAD+ Metabolic Pathways
Sequential activation
Product Data
Compound Identity
Product NameNAD+ (Nicotinamide Adenine Dinucleotide)
Functional ClassNAD+ Precursor & Sirtuin Activator
FormLyophilized
Purity≥98%
Content1000mg
Count1 capsule
Research UseFor in vitro and laboratory research use only. Not for human consumption.
Specifications
Technical Specs
CAS Number53-84-9
Molecular Weight663.43 g/mol
Molecular FormulaC21H27N7O14P2
PubChem CID5892
AppearanceWhite to off-white powder
Storage–20°C / Protect from light and moisture
Formulation Reference
Anatomy of a Peptide
A reference guide to the components of a lyophilized research peptide — from the active sequence to the excipients, solvents, buffers, and stabilizers used in formulation.
Active Peptide 2 items
Synthetic Amino Acid Sequence
The primary chain of amino acids synthesized via solid-phase peptide synthesis (SPPS). Defined by sequence length and molecular weight.
Peptide Modifications
Acetylation (N-terminus), amidation (C-terminus), PEGylation, or cyclization applied to improve stability, receptor binding, or half-life.
Excipients 4 items
Mannitol
Sugar alcohol bulking agent that forms an elegant lyophilized cake, aids reconstitution, and provides structural matrix during freeze-drying.
Trehalose
Non-reducing disaccharide that stabilizes peptide secondary structure by replacing water molecules through hydrogen bonding during dehydration.
Sucrose
Disaccharide used as a lyoprotectant and tonicity agent. Forms an amorphous glassy matrix that immobilizes the peptide and prevents aggregation.
Glycine
Amino acid bulking agent used in lyophilization. Crystallizes to provide mechanical strength to the freeze-dried cake structure.
Reconstitution Solvents 4 items
Bacteriostatic Water (BAC Water)
Sterile water containing 0.9% benzyl alcohol as a preservative. Preferred for multi-dose vials — inhibits microbial growth after initial puncture.
Sterile Water for Injection
USP-grade water, pyrogen-free, without preservatives. Used for single-dose preparations or when benzyl alcohol sensitivity is a concern.
Acetic Acid Solution (0.1–1%)
Dilute acid used for peptides with poor aqueous solubility at neutral pH. Protonates basic residues to improve dissolution.
Sodium Chloride 0.9%
Isotonic saline diluent. Provides physiological osmolality (~308 mOsm/L) and can improve stability of certain charged peptides.
Buffer Systems 4 items
Phosphate Buffered Saline (PBS)
Maintains pH 7.2–7.4. Composed of sodium phosphate dibasic, potassium phosphate monobasic, NaCl, and KCl. Mimics physiological ionic strength.
Acetate Buffer
Effective pH range 3.7–5.6. Composed of acetic acid and sodium acetate. Ideal for acidic peptides and those requiring lower pH for solubility.
Citrate Buffer
Effective pH range 3.0–6.2. Offers strong buffering capacity and metal-chelating properties. Used when oxidation-sensitive residues (Met, Cys) are present.
Histidine Buffer
Effective pH range 5.5–7.0. Low ionic strength, minimal interaction with peptides. Increasingly preferred in modern biopharmaceutical formulations.
Lyoprotectants & Cryoprotectants 3 items
Trehalose / Sucrose (Lyoprotectant)
Protect peptide conformation during the drying phase of lyophilization by forming hydrogen bonds that substitute for water molecules around the peptide.
Glycerol (Cryoprotectant)
Polyol that depresses the freezing point and reduces ice crystal formation, preventing mechanical damage to peptide structure during freezing steps.
Polyethylene Glycol (PEG)
Hydrophilic polymer that provides steric stabilization, reduces aggregation, and can serve as both cryoprotectant and solubility enhancer.
Preservatives & Antimicrobials 3 items
Benzyl Alcohol (0.9%)
Aromatic alcohol preservative in bacteriostatic water. Acts as antimicrobial agent by disrupting microbial cell membranes. Standard for multi-use vials.
Methyl / Propyl Parabens
Broad-spectrum antimicrobial preservatives effective against fungi and bacteria. Used in some peptide formulations where benzyl alcohol is incompatible.
Phenol (0.5%)
Bacteriostatic preservative used in certain injectable peptide formulations. Also acts as a conformational stabilizer for some peptide structures.
Counter Ions & Salt Forms 3 items
Trifluoroacetate (TFA)
Most common counter ion from RP-HPLC purification. Forms TFA salt with basic residues (Lys, Arg, His). May affect bioassay results and cell toxicity.
Acetate
Milder alternative to TFA obtained via ion exchange. Lower cytotoxicity, preferred for cell-based research assays and in vivo studies.
Hydrochloride (HCl)
Chloride salt form, sometimes used for improved stability or specific solubility profiles. Common in pharmaceutical-grade peptide preparations.
Chelating Agents 2 items
EDTA (Disodium)
Chelates divalent metal ions (Cu²⁺, Fe²⁺, Zn²⁺) that catalyze oxidative degradation of methionine and cysteine residues in peptides.
Citric Acid
Natural chelator with moderate metal-binding capacity. Dual function as buffer component and oxidation inhibitor in peptide formulations.
Antioxidants & Stabilizers 3 items
L-Methionine
Free methionine added as a sacrificial antioxidant. Preferentially oxidizes before methionine residues within the peptide chain.
Ascorbic Acid
Water-soluble antioxidant that scavenges reactive oxygen species. Used at low concentrations to prevent oxidative peptide degradation.
Polysorbate 20 / 80
Non-ionic surfactants that prevent surface adsorption and aggregation of peptides at air-liquid and container-liquid interfaces.
Preparation Tool
Reconstitution Calculator
Enter your target working concentration to calculate the exact solvent volume needed for this vial.
mg
Recommended solvents
Bacteriostatic Water Sterile Water for Injection Acetic Acid 0.1% Sodium Chloride 0.9%
Product Specs
Solubility Profile
WaterHighly soluble
Acidified WaterHighly soluble
DMSOHighly soluble
EthanolModerate
Lipid solventsPoor compatibility
Product Specs
Storage Specs
Lyophilized2–8°C preferred
Long-term−20°C recommended
Light SensitivityModerate
MoistureHigh sensitivity
StabilityStable when dry
ContainerSterile sealed vial
Literature
Research Citations
[1]Bhasin S, Seals D, Migaud M, Musi N, Baur JA. Nicotinamide Adenine Dinucleotide in Aging Biology: Potential Applications and Many Unknowns. Endocr Rev. 2023;44(6):1047-1073.
[2]Imai S, Guarente L. NAD+ and sirtuins in aging and disease. Trends Cell Biol. 2014;24(8):464-471.
[3]Massudi H, Grant R, Braidy N, Guest J, Farnsworth B, Guillemin GJ. Age-associated changes in oxidative stress and NAD+ metabolism in human tissue. PLoS One. 2012;7(7):e42357.
[4]Elhassan YS, Kluckova K, Fletcher RS, Schmidt MS, Garten A, Doig CL, et al. Nicotinamide Riboside Augments the Aged Human Skeletal Muscle NAD(+) Metabolome and Induces Transcriptomic and Anti-inflammatory Signatures. Cell Rep. 2019;28(7):1717-1728.e6.
[5]Camacho-Pereira J, Tarragó MG, Chini CCS, Nin V, Escande C, Warner GM, et al. CD38 Dictates Age-Related NAD Decline and Mitochondrial Dysfunction through an SIRT3-Dependent Mechanism. Cell Metab. 2016;23(6):1127-1139.
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Important Notice
Research Use Only

AminoBox products are supplied for research, analytical, and laboratory use only. Product information is provided for educational and technical reference and does not constitute medical advice. Products are not intended to diagnose, treat, cure, or prevent any disease.

Product Composition

Property Specification
Product Name NAD+
Full Name Nicotinamide Adenine Dinucleotide
Compound Content 1000mg
Compound Class Dinucleotide coenzyme
Physical Form Lyophilized powder or sterile solution
Appearance White to off-white powder
Purity Typically ≥98–99%
Research Category Cellular energy & mitochondrial research

Molecular Information

Property Specification
Molecular Formula C21H27N7O14P2
Molecular Weight 663.43 g/mol
CAS Number 53-84-9
PubChem CID 5893
Compound Type Oxidized coenzyme
Biological Classification Pyridine nucleotide cofactor
Related Forms NADH, NADP+, NADPH

NAD+ is the oxidized form of nicotinamide adenine dinucleotide and functions as a critical electron carrier in cellular metabolism.

Structural Classification

Category Description
Compound Type Dinucleotide coenzyme
Functional Class Electron transfer cofactor
Biological Focus Mitochondrial and metabolic signaling research
Mechanistic Focus Cellular redox and ATP production pathways
Chemical Family Pyridine nucleotide

Mechanism Research Profile

Research Focus Description
Mitochondrial Function Investigated in ATP and oxidative phosphorylation pathways
Cellular Energy Studied as a core metabolic cofactor
Redox Signaling Explored in electron transport and oxidation-reduction reactions
DNA Repair Investigated in PARP and sirtuin-associated pathways
Cellular Stress Response Studied in metabolic adaptation and resilience models

Research literature commonly associates NAD+ with mitochondrial energy production, cellular metabolism, and redox biology.

Research Areas Commonly Associated

Research Area Focus
Longevity Biology Cellular aging and resilience pathways
Mitochondrial Research ATP production and energy metabolism
Cognitive Research Neuronal energy signaling
Metabolic Research Glucose and fatty acid metabolism
Cellular Repair Research DNA repair and stress response pathways

Solubility Profile

Solvent Solubility
Water Highly soluble
PBS Buffer Soluble
Sterile Water Compatible
Bacteriostatic Water Compatible for laboratory preparation

NAD+ is generally characterized as highly water soluble under laboratory conditions.

Storage Specifications

Parameter Recommendation
Lyophilized Storage -20°C preferred
Refrigerated Storage 2–8°C after reconstitution
Light Sensitivity Moderate
Moisture Sensitivity High
Stability Stable in dry lyophilized form
Container Type Sterile amber vial

Technical Characteristics

Feature Notes
Delivery Format Lyophilized powder or sterile solution
Biological Role Electron carrier coenzyme
Oxidation State Oxidized NAD form
Hydrophilicity Highly hydrophilic
Stability Profile Sensitive to heat and prolonged moisture exposure
Research Use Laboratory research only

Structurally, NAD⁺ is composed of two nucleotides joined through their phosphate groups:

  • One adenine-containing nucleotide (adenosine monophosphate)
  • One nicotinamide-containing nucleotide (nicotinamide mononucleotide)

This dinucleotide configuration enables to exist in a dynamic equilibrium between oxidized (NAD⁺) and reduced (NADH) states, forming the basis of its function in electron transfer reactions.

Core Biochemical Function: Redox Coupling and Energy Metabolism

NAD⁺ functions as a primary electron acceptor in metabolic oxidation-reduction reactions. It is central to the conversion of macronutrients into usable cellular energy via interconnected biochemical pathways.

Key metabolic roles include:

  • Glycolytic oxidation reactions (cytosolic NAD⁺ → NADH conversion)
  • Tricarboxylic acid (TCA/Krebs) cycle electron capture
  • β-oxidation of fatty acids
  • Oxidative phosphorylation coupling via mitochondrial electron transport chain

In its oxidized form (NAD⁺), the molecule accepts hydride ions (H⁻), forming NADH. This reduced form subsequently donates electrons to Complex I of the mitochondrial electron transport chain, driving proton gradient formation and ATP synthesis.

This continuous cycling between NAD⁺ and NADH constitutes one of the most fundamental energy transduction systems in biological chemistry.

Enzymatic Cofactor Role and Class-Specific Interactions

Beyond its role in redox reactions, NAD⁺ serves as an essential substrate for multiple enzyme families, particularly those involved in post-translational modifications and genomic regulation.

1. Sirtuin Enzymes (Class III Histone Deacetylases)

NAD⁺ is a required co-substrate for sirtuin activity. Sirtuins catalyze NAD⁺-dependent deacetylation reactions on histone and non-histone proteins, linking metabolic state directly to chromatin architecture and transcriptional control.

This establishes NAD⁺ as a metabolic regulator of epigenetic expression patterns.

2. PARP Enzymes (Poly-ADP-Ribose Polymerases)

PARP enzymes consume NAD⁺ to synthesize poly-ADP-ribose chains in response to DNA strand breaks. This process is essential in:

  • DNA damage sensing
  • Base excision repair pathways
  • Genomic stability maintenance

NAD⁺ availability directly influences cellular capacity for DNA repair signaling throughput.

3. CD38/CD157 Ectoenzyme Systems

CD38 functions as a major NAD⁺ hydrolase, catalyzing the conversion of NAD  into cyclic ADP-ribose, a secondary messenger involved in intracellular calcium signaling dynamics.

This pathway positions NAD⁺ as a precursor to calcium-dependent signal transduction networks.

Cellular Compartmentalization and Transport Dynamics

NAD⁺ is compartmentalized across distinct cellular regions, each with independent NAD pools:

  • Mitochondrial NAD pool: drives oxidative phosphorylation and TCA cycle flux
  • Cytosolic NAD pool: regulates glycolytic throughput and biosynthetic reactions
  • Nuclear NAD  pool: supports DNA repair and chromatin remodeling processes

Notably, NAD  does not freely diffuse across mitochondrial membranes; instead, it relies on shuttle systems such as:

  • Malate-aspartate shuttle
  • Glycerol-3-phosphate shuttle

This compartmental separation creates functionally distinct NAD⁺ microenvironments with independent redox ratios (NAD⁺/NADH).

Systems Biology and Metabolic Network Integration

A central node in metabolic network topology, functioning as both:

  1. A redox cofactor in catabolic energy extraction
  2. A signaling substrate in regulatory enzyme systems

This dual role places NAD⁺ at the intersection of:

  • Energy metabolism
  • Epigenetic regulation
  • DNA repair fidelity systems
  • Calcium signaling cascades
  • Mitochondrial biogenesis regulation pathways

Systems biology analyses demonstrate that fluctuations in availability can propagate through multiple biochemical layers, influencing transcriptional networks, mitochondrial efficiency, and enzymatic activity profiles.

Age-Associated NAD⁺ Decline and Metabolic Drift

A substantial body of biochemical literature documents a progressive decline in intracellular NAD⁺ concentrations with biological aging. This decline is associated with:

  • Increased CD38-mediated NAD⁺ consumption
  • Reduced biosynthetic pathway efficiency (NAMPT-mediated salvage pathway decline)
  • Accumulation of DNA damage increasing PARP consumption demand
  • Mitochondrial dysfunction and redox imbalance

The resulting shift in NAD⁺/NADH ratio is considered a key marker of cellular metabolic drift and bioenergetic inefficiency in aging systems.

Biosynthetic Pathways and Metabolic Recycling

NAD⁺ is continuously synthesized and recycled through three primary pathways:

1. Salvage Pathway (Primary Route)

Recycling of nicotinamide via NAMPT-mediated conversion back into NMN and subsequently NAD⁺.

2. De Novo Pathway

Synthesis from tryptophan via the kynurenine metabolic pathway, involving multiple enzymatic intermediates.

3. Preiss-Handler Pathway

Utilization of nicotinic acid (niacin) as a precursor substrate.

The salvage pathway is considered the dominant contributor to intracellular NAD⁺ homeostasis under physiological conditions.

Redox Ratio Significance (NAD⁺/NADH)

The NAD⁺/NADH ratio is a critical determinant of cellular metabolic state:

  • High NAD⁺/NADH ratio → oxidative metabolic dominance, increased mitochondrial flux
  • Low NAD⁺/NADH ratio → reductive stress, impaired electron transport efficiency

This ratio acts as a metabolic rheostat controlling energy system directionality and enzymatic throughput efficiency.

Scientific Reference Table

Research Focus Key Study Link
NAD⁺ metabolism and aging biology Verdin, Hirschey, et al. NAD⁺ in aging and disease https://pubmed.ncbi.nlm.nih.gov/27188365/
Sirtuin activation and NAD⁺ dependence NAD⁺-dependent deacetylation mechanisms https://pubmed.ncbi.nlm.nih.gov/20090218/
DNA repair and PARP-NAD⁺ consumption PARP enzymes and NAD⁺ depletion dynamics https://pubmed.ncbi.nlm.nih.gov/19578250/
Mitochondrial NAD⁺ redox control NAD⁺ compartmentalization in mitochondria https://pubmed.ncbi.nlm.nih.gov/24957114/
CD38-mediated NAD⁺ decline in aging CD38 as NAD⁺ hydrolase in age-related decline https://pubmed.ncbi.nlm.nih.gov/30061704/
NAD⁺ biosynthesis pathways overview Salvage and de novo NAD⁺ pathways https://pubmed.ncbi.nlm.nih.gov/28935782/
Systems biology of NAD⁺ metabolism Metabolic network integration of NAD⁺ https://pubmed.ncbi.nlm.nih.gov/31835577/