2000
DOI: 10.1177/002215540004800116
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Novel Application of Tyramide Signal Amplification (TSA): Ultrastructural Visualization of Double-labeled Immunofluorescent Axonal Profiles

Abstract: SUMMARY Fluorescent immunocytochemistry (FICC) allows multiple labeling approaches when enzyme-based techniques are difficult to combine, such as in double-labeling experiments targeting small-caliber axonal segments. Nevertheless, the conversion of FICC to a product visible at the electron microscopic (EM) level requires labor-intensive procedures, thus justifying the development of more user-friendly conversion methods. This study was initiated to simplify the conversion of FICC to EM by employing the unique… Show more

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Cited by 19 publications
(11 citation statements)
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“…Our findings for RMO14 and SBDP150 run counter to the observation that axons typically label for both markers in studies on rats examined 15 min to 3 h after TBI induced by moderate impact acceleration (Buki et al, 1999, 2000). It is likely that responses to different types and magnitudes of injury follow different time courses, with moderate impact acceleration TBI probably being more severe than our blast injury and its sequelae transpiring more quickly.…”
Section: Discussioncontrasting
confidence: 99%
See 1 more Smart Citation
“…Our findings for RMO14 and SBDP150 run counter to the observation that axons typically label for both markers in studies on rats examined 15 min to 3 h after TBI induced by moderate impact acceleration (Buki et al, 1999, 2000). It is likely that responses to different types and magnitudes of injury follow different time courses, with moderate impact acceleration TBI probably being more severe than our blast injury and its sequelae transpiring more quickly.…”
Section: Discussioncontrasting
confidence: 99%
“…Although nearly 80% of SBDP+ axonal profiles were RMO14+ by 2 days, the early pathology we observed differs from that produced by moderate impact acceleration, where injured axons exhibit extensive SBDP150 and RMO14 double-labeling within 15 min (Buki et al, 1999, 2000). The latter findings have led to the inference that RMO14 labeling is a consequence of μ-calpain proteolysis of neurofilament sidearms (Buki and Povlishock, 2006).…”
Section: Discussioncontrasting
confidence: 59%
“…For immunofluorescent detection, slides were processed using the tyramide-amplification procedure (Stanarius et al, 1997, Stanarius et al, 1999, Toda et al, 1999, Wang et al, 1999, Buki et al, 2000, Bobrow and Moen, 2001). Briefly, the slides were incubated in affinity-purified rabbit anti-alarin (Santic et al, 2007) as primary antibody (1:100 in KPBS with 0.4% Triton-X) for 24 hr at room temperature.…”
Section: Methodsmentioning
confidence: 99%
“…Secondary antibodies used were FITC-, Rhodamine- or Cy3-conjugated donkey anti-Rabbit and FITC- or Rhodamine-conjugated donkey anti-Goat (all 1:200, Jackson Immuno Research, USA). When two primary antibodies from the same species were used, tyramide amplification combined with sequential immuofluorescence was performed following the technique described in Büki et al (Buki et al, 2000). Fluorescent images were captured using a Fast1394 QImaging Camera (QImaging, Canada) installed on a Leica Dmi 4000B microscope (Leica, Germany).…”
Section: Methodsmentioning
confidence: 99%