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      Evaluation of Decalcification Techniques for Rat Femurs Using HE and Immunohistochemical Staining

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          Abstract

          Aim. In routine histopathology, decalcification is an essential step for mineralized tissues. The purpose of this study is to evaluate the effects of different decalcification solutions on the morphological and antigenicity preservation in Sprague Dawley (SD) rat femurs. Materials and Methods. Four different decalcification solutions were employed to remove the mineral substances from rat femurs, including 10% neutral buffered EDTA, 3% nitric acid, 5% nitric acid, and 8% hydrochloric acid/formic acid. Shaking and low temperature were used to process the samples. The stainings of hematoxylin-eosin (HE) and immunohistochemical (IHC) were employed to evaluate the bone morphology and antigenicity. Key Findings. Different decalcification solutions may affect the quality of morphology and the staining of paraffin-embedded sections in pathological examinations. Among four decalcifying solutions, 3% nitric acid is the best decalcifying agent for HE staining. 10% neutral buffered EDTA and 5% nitric acid are the preferred decalcifying agents for IHC staining. Significance. The current study investigated the effects of different decalcifying agents on the preservation of the bone structure and antigenicity, which will help to develop suitable protocols for the analyses of the bony tissue.

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          When tissue antigens and antibodies get along: revisiting the technical aspects of immunohistochemistry--the red, brown, and blue technique.

          Once focused mainly on the characterization of neoplasms, immunohistochemistry (IHC) today is used in the investigation of a broad range of disease processes with applications in diagnosis, prognostication, therapeutic decisions to tailor treatment to an individual patient, and investigations into the pathogenesis of disease. This review addresses the technical aspects of immunohistochemistry (and, to a lesser extent, immunocytochemistry) with attention to the antigen-antibody reaction, optimal fixation techniques, tissue processing considerations, antigen retrieval methods, detection systems, selection and use of an autostainer, standardization and validation of IHC tests, preparation of proper tissue and reagent controls, tissue microarrays and other high-throughput systems, quality assurance/quality control measures, interpretation of the IHC reaction, and reporting of results. It is now more important than ever, with these sophisticated applications, to standardize the entire IHC process from tissue collection through interpretation and reporting to minimize variability among laboratories and to facilitate quantification and interlaboratory comparison of IHC results.
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            Effects of thirty elements on bone metabolism.

            The human skeleton, made of 206 bones, plays vital roles including supporting the body, protecting organs, enabling movement, and storing minerals. Bones are made of organic structures, intimately connected with an inorganic matrix produced by bone cells. Many elements are ubiquitous in our environment, and many impact bone metabolism. Most elements have antagonistic actions depending on concentration. Indeed, some elements are essential, others are deleterious, and many can be both. Several pathways mediate effects of element deficiencies or excesses on bone metabolism. This paper aims to identify all elements that impact bone health and explore the mechanisms by which they act. To date, this is the first time that the effects of thirty minerals on bone metabolism have been summarized.
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              JiangTang XiaoKe granule attenuates cathepsin K expression and improves IGF-1 expression in the bone of high fat diet induced KK-Ay diabetic mice

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                Author and article information

                Journal
                Biomed Res Int
                Biomed Res Int
                BMRI
                BioMed Research International
                Hindawi Publishing Corporation
                2314-6133
                2314-6141
                2017
                26 January 2017
                : 2017
                : 9050754
                Affiliations
                1Preclinical Medicine School, Beijing University of Chinese Medicine, Beijing 100029, China
                2Chinese Material Medica School, Beijing University of Chinese Medicine, Beijing 100029, China
                3Diabetes Research Center, Beijing University of Chinese Medicine, Beijing 100029, China
                4The Research Institute of McGill University Health Center, Montreal, QC, Canada H4A 3J1
                5Oral Biological Medicinal Science, University of British Columbia, Vancouver, BC, Canada V6T 1Z3
                Author notes
                *Dongwei Zhang: dongwei1006@ 123456gmail.com and

                Academic Editor: Alexander N. Orekhov

                Author information
                http://orcid.org/0000-0002-0757-984X
                http://orcid.org/0000-0002-7793-1482
                http://orcid.org/0000-0002-0332-3767
                Article
                10.1155/2017/9050754
                5299168
                28246608
                0e057fa5-ec5d-4061-8736-db8b30888aeb
                Copyright © 2017 Haixia Liu et al.

                This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

                History
                : 16 November 2016
                : 20 December 2016
                Funding
                Funded by: National Natural Science Foundation of China
                Award ID: NSFC81274041
                Award ID: NSFC81273995
                Funded by: MOE
                Award ID: 2011DFA30920
                Award ID: B07007
                Funded by: MOST
                Award ID: 20122X09103201-005
                Categories
                Research Article

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