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(Top) 1 Procedure 2 Combination methods 3 See also 4 References

Luxol fast blue stain

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Micrograph of the pons using a hematoxylin & eosin-luxol fast blue stain.

Coronal section of a mouse brain stained with Hematoxylin & LFB

Luxol fast blue stain, abbreviated LFB stain or simply LFB, is a commonly used stain to observe myelin under light microscopy, created by Heinrich Klüver and Elizabeth Barrera in 1953.^[1] LFB is commonly used to detect demyelination in the central nervous system (CNS), but cannot discern myelination in the peripheral nervous system.^[2]

Procedure[edit]

Luxol fast blue is a copper phthalocyanine dye that is soluble in alcohol and is attracted to bases found in the lipoproteins of the myelin sheath.^[3]^[4]

Under the stain, myelin fibers appear blue, neuropil appears pink, and nerve cells appear purple. Tissues sections are treated over an extended period of time (usually overnight) and then differentiated with a lithium carbonate solution.^[4]

Combination methods[edit]

The combination of LFB with a variety of common staining methods provides the most useful and reliable method for the demonstration of pathological processes in the CNS.^[2] It is often combined with H&E stain (hematoxylin and eosin), which is abbreviated H-E-LFB, H&E-LFB. Other common staining methods include the periodic acid-Schiff, Oil Red O, phosphotungstic acid, and Holmes silver nitrate method.^[2]

References[edit]

^ Kluver H., Barrera E. (1953). "A method for the combined staining of cells and fibers in the Nervous system". J. Neuropathol. Exp. Neurol. 12 (4): 400–403. doi:10.1097/00005072-195312040-00008. PMID 13097193.

^ ^a ^b ^c Shin J. Oh (2002). Color Atlas of Nerve Biopsy Pathology. CRC Press. pp. 191–. ISBN 978-0-8493-1676-0. Retrieved 1 January 2013.

^ Bruce-Gregorios, Jocelyn (2006). Histophatologic Techniques. Goodwill Trading Co., Inc. pp. 241–. ISBN 978-971-12-0270-5. Retrieved 1 January 2013.

^ ^a ^b Peter A. Humphrey; Louis P. Dehner; John D. Pfeifer (2008). The Washington Manual of Surgical Pathology: Department of Pathology and Immunology, Washington University School of Medicine, St. Louis, Missouri. Lippincott Williams & Wilkins. pp. 681–. ISBN 978-0-7817-6527-5. Retrieved 1 January 2013.

v t e Microbial and histological stains
Iron/hemosiderin	Perls Prussian blue
Lipids	Sudan stain Sudan II Sudan III Sudan IV Oil Red O Sudan Black B
Carbohydrates	Alcian blue Mucicarmine Periodic acid–Schiff stain
Amyloid	Congo red Thioflavin
Bacteria	Gram stain Methyl violet/Gentian violet Safranin Acid-fast Ziehl–Neelsen stain/Kinyoun stain Carbol fuchsin/Fuchsine Methylene blue Auramine–rhodamine stain Auramine O Rhodamine B Auramine phenol stain
Connective tissue	trichrome stain: Masson's trichrome stain/Lillie's trichrome Light Green SF yellowish Biebrich scarlet Phosphomolybdic acid Fast Green FCF Sirius Red Van Gieson's stain
Other	Cresyl violet Cyanine Jaswant Singh–Bhattacharji (JSB) stain H&E stain Haematoxylin Eosin Y Janus Green B Giemsa stain Gömöri trichrome stain Luxol fast blue stain Methyl blue Moeller stain Movat's stain Neutral red Schaeffer–Fulton stain Silver stain Bielschowsky stain Grocott's methenamine silver stain Warthin–Starry stain Wright's stain
Tissue stainability	Acidophilic Basophilic Chromophobic

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