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  3. Sudan IV

Sudan IV  (Synonyms: Solvent Red 24; C.I. 26105)

Cat. No.: HY-D0932 Purity: ≥98.0%
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Sudan IV is an agonist of the aryl hydrocarbon receptor (AhR) that activates downstream signaling pathways and induces CYP1A1 expression. Sudan IV promotes CYP1A1 gene transcription by activating AhR-ARNT heterodimers and binding to exogenous response elements (XREs) on DNA, thereby enhancing drug metabolizing enzyme activity. Sudan IV can be used to study the toxicity mechanisms of industrial dyes and the effects of interactions with serum proteins (such as bovine serum albumin (BSA)) on their distribution in vivo. Sudan IV is a fat-soluble diazo dye that can be used to stain lipids, triglycerides, and lipoproteins on frozen sections.

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Sudan IV Chemical Structure

Sudan IV Chemical Structure

CAS No. : 85-83-6

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Based on 1 publication(s) in Google Scholar

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Description

Sudan IV is an agonist of the aryl hydrocarbon receptor (AhR) that activates downstream signaling pathways and induces CYP1A1 expression. Sudan IV promotes CYP1A1 gene transcription by activating AhR-ARNT heterodimers and binding to exogenous response elements (XREs) on DNA, thereby enhancing drug metabolizing enzyme activity. Sudan IV can be used to study the toxicity mechanisms of industrial dyes and the effects of interactions with serum proteins (such as bovine serum albumin (BSA)) on their distribution in vivo. Sudan IV is a fat-soluble diazo dye that can be used to stain lipids, triglycerides, and lipoproteins on frozen sections[1][2][3][4].

IC50 & Target

CYP1A1

 

In Vitro

In vitro binding experiment (bovine serum albumin interaction): Sudan IV (1×10-6 M; 30 min) binds to bovine serum albumin (BSA) via van der Waals forces with a binding constant of 1.48×104 M-1, resulting in a decrease in the α-helical structure and an increase in the β-fold of BSA, inducing a conformational change in the protein[2].
Fluorescence detection experiment (Cu2+-calcein system): The fluorescence of calcein can be effectively quenched by Cu(II). During the ligand exchange reaction, Sudan I and Sudan III can capture the Cu(II) on calcein, resulting in the recovery of calcein fluorescence. Sudan IV (6.06×10-7 M; 90 min) is unable to bind to Cu2+ and displace calcein, resulting in no significant recovery of the fluorescence intensity of the Cu2+-calcein complex[3].

Sudan IV Cryosection Staining Protocol[4]
Materials
Fresh or cryopreserved tissue (e.g., liver transplant donor tissue) was cut into 8-micron-thick frozen sections.
Sudan staining solution: a mixture of 50% Sudan IV dye (Sigma Aldrich) and 50% Sudan III dye (volume ratio), stored at room temperature.
Hematoxylin staining solution: used for counterstaining of cell nuclei.
Aqueous mounting medium: used for section sealing.
Equipment: Cryostat, optical microscope (Zeiss Axio A10), digital camera (Axio Cam 506), staining jar, slide.
Operation steps
Slice preparation: Use a cryostat to cut the tissue into 8 μm thick slices and attach them to slides (the thickness of the slices is clearly stated in the document to be 8 μm). Avoid repeated freezing and thawing to keep the slices fresh to preserve the lipid structure.
Staining: Immerse the slices in Sudan IV staining solution (can be used alone or mixed with Sudan III in equal proportions) and stain at room temperature for 10 minutes (the mixed staining time in the document is 10 minutes). Rinse quickly with distilled water once to remove excess stain on the surface (avoid excessive rinsing that may cause stain loss).
Counter-stain cell nuclei: Immerse in hematoxylin staining solution and counter-stain at room temperature for 1-2 minutes to make the cell nuclei appear blue. Rinse twice with distilled water for 30 seconds each to remove excess hematoxylin.
Seal and observe: Add aqueous sealant to the slice surface and cover with a glass slide to avoid bubbles. Observe immediately under an optical microscope (100×, 200×, 400× magnifications are used in the document) and take digital images for subsequent analysis (such as machine learning algorithm to quantify fat vacuoles).
Staining results
Fat vacuoles: Orange or orange-red vacuoles can be seen inside the cell.
Cell nucleus: blue, located at the edge of the cell or squeezed and displaced by fat vacuoles.
Background: No specific staining, cytoplasm and non-fat structures are light or colorless.
Precautions
Storage of staining solution: Sudan IV is a fat-soluble dye, and the staining solution needs to be sealed to prevent solvent evaporation from affecting the staining effect.
Slice thickness: Strictly control the slice thickness to 8 μm. Too thick may cause uneven staining, and too thin may cause tissue damage.
Re-staining time: The hematoxylin re-staining time should not be too long to avoid too dark background affecting the identification of fat vacuoles.
Image analysis: Images should be taken as soon as possible after staining to avoid dye fading; machine learning algorithms (such as KNN, Naive Bayes) can be combined to quantify the proportion of fat vacuoles.

MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only.

In Vivo

Rat liver CYP1A1 induction: Sudan IV (40 mg/kg; intraperitoneal injection, 3 days) induces the mRNA and protein expression of cytochrome P450 1A1 (CYP1A1) in the Wistar rat model, with an induction capacity of 2/3 that of Sudan III. Immunohistochemistry showed that CYP1A1 was dominantly distributed in the perihilar region of liver tissue[1].

MedChemExpress (MCE) has not independently confirmed the accuracy of these methods. They are for reference only.

Molecular Weight

380.44

Formula

C24H20N4O

CAS No.
Appearance

Solid

Color

Light brown to brown

SMILES

OC1=CC=C2C=CC=CC2=C1/N=N/C3=CC=C(/N=N/C4=CC=CC=C4C)C=C3C

Shipping

Room temperature in continental US; may vary elsewhere.

Storage
Powder -20°C 3 years
4°C 2 years
In solvent -80°C 6 months
-20°C 1 month
Solvent & Solubility
In Vitro: 

DMSO : < 1 mg/mL (insoluble or slightly soluble)

*Sudan IV is usually formulated as a suspension.

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Purity & Documentation
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  • Do most proteins show cross-species activity?

    Species cross-reactivity must be investigated individually for each product. Many human cytokines will produce a nice response in mouse cell lines, and many mouse proteins will show activity on human cells. Other proteins may have a lower specific activity when used in the opposite species.

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Sudan IV
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