Characterization of the human syncytiotrophoblast plasma membrane associated components

We have studied the mechanisms involved in calcium (Ca2+) transport through the basal plasma membranes (BPM) of the syncytiotrophoblast cells from full-term human placenta. These purified membranes were enriched 25-fold in Na+/ K+-adenosine triphosphatase (ATPase), 37-fold in [3H]dihydroalprenoloI b

The plasma membranes from ejaculated human spermatozoa were removed by nitrogen cavitation (600 PSI for 10 min) and isolated by centrifugation followed by a discontinuous sucrose density gradient centrifugation. Glycolipid analysis of the plasma membrane revealed a three-fold enrichment in gangliosi

Ejaculated human spermatozoa were subjected to nitrogen cavitation (600 psi for ten min) to remove the plasma membrane (PM). Electron microscopic examination of the cavitated cells revealed that 33% of the PM was removed from the sperm which includes both the head and tail regions. The released memb

## Abstract Externally oriented components on the human sperm cell surface and components in human seminal plasma were labeled by enzymatic iodination with lactoperoxidase and [^125^I] NaI. SDS‐7.5% PAGE of labeled sperm surface resolved one minor and four major components with approximate molecula

## Abstract The surface proteins of seven human cell lines (three bladder carcinomas (TCC), two normal urothelial lines, one colon carcinoma, and one malignant melanoma) were labelled with ^125^I by the glucose oxidase‐lactoperoxidase technique. Plasma membranes of the cells were isolated and analy

## Abstract The role of α‐actinin in the attachment of actin to plasma membranes has been investigated. Specific antibody staining of SDS gels has indicated that α‐actinin is a major component in isolated plasma membranes prepared from three different cell types by two different procedures. Using s