IHC: 10 µg/ml, membrane permeabilization (acetone) is essential. The antibody Hs-14 is designed for quantitative immunofluorescence analysis of pathological sperms (excellent tool for laboratories of assisted reproduction when optimal method of fertilization is sought), Flow Cytometry: Intraacrosomal staining: 3-12 µg/ml.

Reaktivität

Mouse, Human

Immunogen

Freshly ejaculated human sperms were washed in PBS and extracted in 3% acetic acid, 10% glycerol, 30 mM benzaminidine. The acid extract was dialyzed against 0.2% acetic acid and subsequently used for immunization.

Wirt

Mouse

Klonalität

Monoclonal

Klon

Hs-14

Isotyp

IgM

Konjugat

Unconjugated

Reinigung

Purified by differential precipitation and solid-phase chromatography.

Konzentration

1 mg/ml

Geschätztes MW

220 kDa

Produktform

Liquid

Formulierung

Supplied in Tris Buffered Saline, pH 8, with 15 mM Sodium Azide.

Lagerung

Shipped at 4°C. Store at 2-8°C. Do not freeze!

Synonyme

15S Mg(2+) ATPase p97 subunit, 15S Mg(2+)-ATPase p97 subunit, ALS14, ATPase p97, CDC48, IBMPFD, MGC131997, MGC148092, MGC8560, p97, TER ATPase, TERA, TERA_HUMAN, Transitional endoplasmic reticulum ATPase, Valosin containing protein, Valosin-containing protein, Yeast Cdc48p homolog

Isotyp-Kontrollantikörper

Mouse IgM [PRF-03] (A86761)

Kompatible Sekundärantikörper

Haftungsausschluss

Dieses Produkt ist nur für Forschungszwecke bestimmt. Es ist nicht für diagnostische oder therapeutische Zwecke bestimmt.

Produktbilder (1)

Bild Vergrößern

Figure 1: Immunocytochemistry - Anti-VCP Antibody [Hs-14] (A86576)

Immunofluorescence analysis of VCP in acetone-permeabilized human sperms using Anti-VCP Antibody (A86576) demonstrates its location to the acrosome. (Normal spermiogram shown).

Produktreferenzen für diesen Klon (1)

Publikation anzeigen

The use of immunofluorescence in microdissection testicular sperm extraction.

Verweise: Anti-VCP Antibody [Hs-14] (NB500-455)

Abstrakt:

Microdissection testicular sperm extraction (TESE) has been used in the treatment of male infertility in cases of nonobstructive azoospermia (NOA). In some NOA cases, there is significant difficulty identifying sperm within the testes, and we propose that an immunofluorescence technique may assist in locating sperm foci for use in in vitro fertilization and intracytoplasmic sperm injection. The purpose of this study was to evaluate the feasibility of this novel technique. Thirteen fertile and 8 sterile mice were anesthetized, and a lower abdominal incision was performed to deliver the testes. Then a small incision was made into the tunica albuginea near the vascular pedicle to expose the seminiferous tubules. A microinjector fitted with a micropipette was used to inject fluorescein isothiocyanate-conjugated mouse anti-human acrosomal IgM antibody (HS-14) into adjacent injection sites along the exposed seminiferous tubules. Following antibody injection, the testes were examined under a Bio-Rad Multiphoton microscope to locate sperm through visualization of fluorescence. Sperm were identified in 22 of 26 testes from fertile mice either by morphologic appearance or by their motility, which was obvious under direct visualization. There was strong binding of the antibody to both the sperm head and tail. In contrast, no sperm were visualized in the sterile mice group. Use of an immunofluorescence technique during microdissection TESE for detection of sperm is a novel and feasible concept. Further studies of this technique are planned.

Publikation anzeigen