Validation of the bovine blood calcium checker as a rapid and simple measuring tool for the ionized calcium concentration in cattle.

Point-of-care (POC) devices that veterinary practitioners can use to easily and rapidly measure blood ionized calcium (iCa) levels in cows immediately after withdrawing a blood sample on the dairy farm are needed. Aims of present studies was to compare the commercially available ion-selective electrode handheld iCa meter (bovine blood iCa checker) with the benchtop blood gas analyzer GEM premier 3500 and handheld analyzer i-STAT 1. Sixty-two paired-point whole blood samples were obtained from three cows with hypocalcemia experimentally induced by Na2-EDTA infusion. Whole blood samples were also obtained from the 36 cows kept on a farm in field conditions. The results using the bovine blood iCa checker correlated with those using the GEM premier 3500 and i-STAT 1. Bovine blood iCa checker was "compatible" with the GEM premier 3500 and i-STAT 1 because the frequency of differences between the measurements within ± 20% of the mean were 100% (65/65, >75%) and 90.8% (59/65, >75%), respectively. In the field trial, the blood iCa concentration measured by the bovine blood Ca checker was significantly positively correlated with that measured by the i-STAT 1 portable analyzer. Bovine blood iCa checker was "compatible" with the i-STAT 1 because the frequency of differences between the measurements within ± 20% of the mean was 100% (36/36, >75%). Results from these findings, the bovine blood iCa checker may be applied as a simplified system to measure the iCa concentration in bovine whole blood.

Micelle formation of sodium hyodeoxycholate.

Sodium hyodeoxycholate (NaHDC) is the main component of hog bile salts, which play a role in the absorption of sparingly soluble materials in the intestinal solution. The biosurfactant has an amphiphilic molecular structure, similar to that of ursodeoxycholate from bear gallbladder. Micelle formation from hyodeoxycholate was studied at 308.2K using pyrene fluorescence probe to determine critical micelle concentrations (cmc) at various NaCl concentrations. The change in the fluorescence spectrum peak ratios with NaHDC concentration indicated two steps for bile salt aggregation. The first step was the formation of small micelles (cmc) at 5mM, and the second step was the formation of stable aggregates at 14 mM in aqueous solution. The aggregation of hyodeoxycholate, analyzed using the stepwise association model, was found to grow its aggregation number from 4 to 7 with increasing concentration. The aggregation number in aqueous solution was also confirmed by the static light scattering method. The average measured aggregation number of the micelles was 6.7. The micellar size was relatively small as measured by either method, but it was covered by general aggregation number of human bile salts. The degree of counterion binding to the micelles, determined using a sodium ion-selective electrode, was ca. 0.5 for the NaHDC micelles. This value was relatively high among typical bile salts. Moreover, the solubilization capacity of the NaHDC micelles was assessed using cholesterol. It became clear that NaHDC micelles hardly solubilized cholesterol compared to typical human bile salts. The maximum solubilization by NaHDC was equivalent only to that by sodium ursodeoxycholate.