Literature DB >> 13892901

An electron microscope study of the fine structure of feather keratin.

B K FILSHIE, G E ROGERS.   

Abstract

Thin sections of the rachis of regenerating follicles of pigmented fowl feathers and of mature non-pigmented seagull feather rachis, embedded in methacrylate and Araldite respectively, were studied in the electron microscope. The late stages of development of keratin fibrils were examined in OsO(4)-fixed follicle material, and after poststaining with lead hydroxide the keratin aggregates were found to be composed of fine microfibrils approximately 30 A in diameter apparently embedded in a matrix material which had absorbed the lead stain. The centre-to-centre separation of the microfibrils was of the order of 35 A. After bulk treatment by reduction with thioglycollic acid, OsO(4) staining, and poststaining with lead hydroxide, a similar microfibrillar fine structure was observed in mature rachis. Only after lead staining could the microfibrils be delineated, and their diameter and separation were similar to that found in the keratin of the follicle. It is suggested that feather keratin resembles alpha-keratins in consisting of microfibrils embedded in an amorphous protein matrix. However, in comparison with alpha-keratins, the microfibrils are much smaller in diameter, their arrangement is less orderly, and on the basis of the reactions towards the electron staining procedures, the cystine content of the matrix appears to be not greatly different from that of the microfibrils. The significance of a microfibrillar constitution of feather keratin is discussed in relation to current structural models for this fibrous protein deduced from x-ray diffraction studies. The boundaries between the component cells of feather rachis are desmosomal in character and similar to those of related keratinous structures and a number of different types of cells; the melanin granules are dissimilar to those of mammalian epidermis in their apparent lack of melanin-protein lamellae.

Entities:  

Keywords:  BIRDS; KERATIN; MICROSCOPY, ELECTRON

Mesh:

Substances:

Year:  1962        PMID: 13892901      PMCID: PMC2106060          DOI: 10.1083/jcb.13.1.1

Source DB:  PubMed          Journal:  J Cell Biol        ISSN: 0021-9525            Impact factor:   10.539


  13 in total

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2.  A new embedding medium for electron microscopy.

Authors:  A M GLAUERT; R H GLAUERT; G E ROGERS
Journal:  Nature       Date:  1956-10-13       Impact factor: 49.962

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Journal:  J Biophys Biochem Cytol       Date:  1957-09-25

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Journal:  J Biophys Biochem Cytol       Date:  1960-09

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Journal:  J Biophys Biochem Cytol       Date:  1958-11-25

8.  Electron microscope observations of the melanocyte of the human epidermis.

Authors:  A CHARLES; J T INGRAM
Journal:  J Biophys Biochem Cytol       Date:  1959-08

9.  The electron microscopy of the human hair follicle. II. The hair cuticle.

Authors:  M S BIRBECK; E H MERCER
Journal:  J Biophys Biochem Cytol       Date:  1957-03-25

10.  The fine structure of the interrelationship of cells in the human epidermis.

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Journal:  J Biophys Biochem Cytol       Date:  1958-09-25
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  28 in total

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Journal:  Biochem J       Date:  1964-07       Impact factor: 3.857

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Review 7.  The role of β-sheets in the structure and assembly of keratins.

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9.  Expressed miRNAs target feather related mRNAs involved in cell signaling, cell adhesion and structure during chicken epidermal development.

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10.  [Morphological and biochemical investigations of hairs in inborn errors of amino acid metabolism (author's transl)].

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