Antigen retrieval technique utilizing citrate buffer or urea solution for immunohistochemical demonstration of androgen receptor in formalin-fixed paraffin sections.

Shi, Shan‐Rong; Chaiwun, Benjaporn; Young, Lillian; Côté, Richard J.; Taylor, Clive R.

doi:10.1177/41.11.7691930

Cited by 277 publications

(177 citation statements)

References 11 publications

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“…Coronal serial sections (7 m) were mounted on poly-L-lysine-coated slides (Sigma, St Louis, MO, USA) and allowed to air-dry, for 16 h at 45°C, deparaYnized, rehydrated, and treated for immunocytochemistry, as described before (Calle et al, 2005a). As to the Fos staining, the antigen retrieval method of Shi et al (1993) was used. After deparaYnization, sections were pre-heated in a microwave oven at 90°C in 0.3% tri-sodium citrate buVer (pH.…”

Section: Immunocytochemistrymentioning

confidence: 99%

Effect of starvation on Fos and neuropeptide immunoreactivities in the brain and pituitary gland of Xenopus laevis

Calle

Kozicz

Linden

et al. 2006

General and Comparative Endocrinology

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In mammals complex interactions between various brain structures and neuropeptides such as corticotropin-releasing factor (CRF) and urocortin 1 (Ucn1) underlay the control of feeding by the brain. Recently, in the amphibian Xenopus laevis, CRF-and Ucn1-immunoreactivities were shown in the hypothalamic magnocellular nucleus (Mg) and evidence was obtained for their involvement in food intake. To gain a better understanding of the brain structures controlling feeding in X. laevis, the eVects of 16 weeks starvation on neurones immunoreactive (ir) to Fos and neuropeptides in various brain structures were quantiWed. In the Mg, compared to controls, starved animals showed fewer neurones immunopositive for Fos (¡55.9%), Ucn1 (¡44.0%), cocaine and amphetamine-regulated transcript (CART) (¡94.3%) and metenkephalin (ENK) (¡65.0%), whereas CRF-ir neurones were 2.1 times more numerous. These diVerences were mainly apparent in the ventral part of the Mg, followed by the medial and dorsal part of the nucleus. In the neural lobe of the pituitary gland a 22.5% lower optical density of CART-ir was observed. In the four other brain structures investigated, starvation had diVerent eVects. The dorsomedial part of the suprachiasmatic nucleus showed 5.9 times more NPY-ir cells and in the ventromedial thalamic area a lower number of NPY-ir cells (¡33.6%) was found, whereas the Edinger-Westphal nucleus contained fewer CART-ir cells (¡42.2%); no eVect of starvation was seen in the ventral hypothalamic nucleus. Our results support the hypothesis that in X. laevis, the Mg plays a pivotal role in feeding-related processes and, moreover, that starvation also has neuropeptide-and brain structure-speciWc eVects in other parts of the brain and in the pituitary gland, suggesting particular roles of these structures and their neuropeptides in physiological adaptation to starvation.

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Section: Immunocytochemistrymentioning

confidence: 99%

Effect of starvation on Fos and neuropeptide immunoreactivities in the brain and pituitary gland of Xenopus laevis

Calle

Kozicz

Linden

et al. 2006

General and Comparative Endocrinology

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“…Therefore the accessibility of antigenic epitopes might be limited. Such hindrances may be partially reversed by retrieval techniques like enzyme digestion and microwave oven heating [28][29][30]. To identify a suitable method for antigen retrieval, the effect of pretreatment with enzyme and microwave oven heating was studied in tissues from eight mice in the following three experiments:…”

Section: Gf ¼mentioning

confidence: 99%

A Mouse Model for Slowly Progressive Primary Tuberculosis

et al. 1999

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Mustafa T, Phyu S, Nilsen R, Jonsson R, Bjune G. A Mouse Model for Slowly Progressive Primary Tuberculosis. Scand J Immunol 1999;50:127-136 The progression from primary Mycobacterium tuberculosis infection to disease is usually slow in humans. The aim of this study was to develop and characterize a mouse model for slowly progressive primary tuberculosis, using the intraperitoneal (i.p.) route of infection, and to compare it with our previously described model of latent M. tuberculosis infection. B6D2F1 hybrid mice inoculated with 1.5 × 10 6 colony-forming units (CFUs) of M. tuberculosis H37Rv were followed-up for 70 weeks. Lungs, livers and spleens were examined for bacillary growth, histopathological changes and mycobacterial antigens (MPT64, ManLAM and multiple antigens of M. tuberculosis), by immunohistochemical staining. The infection was found to pass through three distinctive phases. During phase 1, mice were healthy despite development of small granulomas and an increasing number of bacilli in the lungs. During phase 2, mice were unwell but mortality was low. The count of M. tuberculosis and the granuloma size stabilized. The granulomas contained an increasing population of large, vacuolated macrophages. During phase 3, mice became moribund and died rapidly, but the M. tuberculosis count remained relatively stable. The inflammatory infiltrates filled Ϸ 80% of the lung parenchyma and the lesions were not well demarcated. Rapidly progressing inflammation, rather than an increase in the M. tuberculosis count, seems to contribute more to mortality.

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“…It has been demonstrated that the AR technique is a simple and effective enhancement method for immunohistochemistry on archival tissue sections. Two major advantages of AR-IHC are (a) reduction of the detection thresholds of immunohistochemical staining (increased sensitivity) for a wide range of antibodies, and (b) retrieval of some antigens, such as Ki-67, MIB1, ER-1D5, bcl-2, androgen receptor, RB, CD5, CD8, CD35, CD38, CD25, CD45R, CD34, CD68, CD44, CD55, VCAM-1, CGA7 (smooth muscle-specific actin), CD19, and thrombospondin (Grossfeld et al 1996;Cuevas et al 1994;Cattoretti et al 1993;Gown et al 1993a;Leong and Milios 1993;Shi et al 1993bShi et al ,1996, which are otherwise negative even with other unmasking pretreatment. At present the AR-IHC method is being widely used for the detection of ER, PR, MIB1, p53, bcl-2, pRB, and some CD markers on routinely formalin-fixed, paraffin-embedded tissue sections in daily pathological diagnosis (for review and detailed data see Shi et al 1995b).…”

Section: Applicationmentioning

confidence: 99%

“…Furthermore, the toxic effect of metal salts, particularly lead salts, is a major drawback. Therefore, several alternative AR solutions were subsequently developed, such as citrate, Tris and other buffer solutions, and urea (Kawai et al 1994b;Taylor et al 1994a;Gown et al 1993a;Leong and Milios 1993;Shi et al 1993b;Gerdes et al 1992), EDTA or EGTA (Morgan et al 1994), glycine-HCl buffer (Imam et al 1995), and periodic acid (Kwaspen et al 1995).…”

Section: The Effect Of Metal Ions the Chemical Composi-mentioning

confidence: 99%

Antigen Retrieval Immunohistochemistry: Past, Present, and Future

Shi

Côté²,

Taylor

1997

J Histochem Cytochem.

480

331

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SUMMARYThe antigen retrieval (AR) technique, which is predominantly based on hightemperature heating of tissues, is used as a non-enzymatic pretreatment for immunohistochemical staining of formalin-fixed, paraffin-embedded tissue sections. It has been widely applied in pathology and analytical morphology. The existence of a growing body of literature on the AR technique raises a number of interesting issues for the further development of AR. These issues include the use of a "test battery" and the concept of "maximal retrieval" applied to the selection of optimal test protocols for the standardization of AR. (J Histochem Cytochem 45:327-343, 1997)

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Antigen retrieval technique utilizing citrate buffer or urea solution for immunohistochemical demonstration of androgen receptor in formalin-fixed paraffin sections.

Cited by 277 publications

References 11 publications

Effect of starvation on Fos and neuropeptide immunoreactivities in the brain and pituitary gland of Xenopus laevis

Effect of starvation on Fos and neuropeptide immunoreactivities in the brain and pituitary gland of Xenopus laevis

A Mouse Model for Slowly Progressive Primary Tuberculosis

Antigen Retrieval Immunohistochemistry: Past, Present, and Future

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