We have developed a two fluid solar wind model from the Sun to 1 AU. Its basic equations are mass, momentum and energy conservations. In these equations, we include a wave mechanism of heating the corona and accelerating the wind. The two fluid model takes into account the power spectrum of Alfvenic wave fluctuation. Model computations have been made to fit observational constraints such as electron(Te) and proton(Tp) temperatures and solar wind speed(V) at 1 AU. As a result, we obtained physical quantities of solar wind as follows: Te is 7.4 X 10.5 K and density(n) is 1.7 X 107 cm-3 in the corona. At 1 AU Te is 2.1 X 105 K and n is 0.3 cm-3, and V is 511 km s-1. Our model well explains the heating of protons in the corona and the acceleration of the solar wind.

This study was performed to test the cellulose digestibility using the transgenic pigs harboring cellulose degradation gene D (CelD). After delivered offsprings between normal pig and transgenic swine, DNA was isolated from piglets tail for PCR analysis. In first generation, five out of 65 piglets showed CelD positive. Unfortunately, four CelD-positive pigs were died during growing, but one survived pig was used as a transgenic founder to produce F₁ descendents. Among 3 F₁ transgenic pigs produced, one died and the remaining two pigs were used to test the fiber digest efficiency. An assorted feed was composite of 5％ fiber with other ingredients. The feed of 3 kg per day was provided to the pigs including transgenic founders and littermate controls. The manure quantity was measured daily for a month, and all manures were dried for three days to analysis nitrogen, phosphate and fiber concentrations. The fiber digestion efficiencies of the transgenic F₁ pigs showed approximately 10％ higher than those of control pigs. Fiber digestion was not greatly improved in transgenic pigs as it had been expected approximately 30％. Nitrogen concentration of transgenic pig′s manure was slowly decreased compare to the control pigs. Because there were only two transgenic pigs tested, a large number of transgenic pigs may be necessary to obtain more reliable data. Breeding of animals to obtain sufficient transgenic pigs subjected for a further study is on progress. Taken together, this study demonstrated successful production of transgenic pigs with increase of cellulose digestibility in the porcine feed.

The present study were performed to analysis the hematocrit and the red blood cells content into the blood plasma of the transgenic pigs harboring recombinent human erythropoietin gene (rhEPO). Mouse whey acidic protein (mWAP) linked to rhEPO gene was microinjected into pronuclei of porcine one-cell zygotes. After delivered of offspring, PCR analyses identified one mWAP-rhEPO transgenic founder offspring(F/sub 0/). The first generation of transgenic pig (F/sub 0/) harboring mWAP-hEPO appeared to be a male, and the second generation (F₁) pigs were made by natural mating of F/sub 0/ with domestic swine, and male and female transgenic pigs (F₁) were identified by PCR. The blood samples from transgenic and normal pigs were collected for 50 days during lactation and were counted the red blood cell (RBC) numbers and Hematocrit (HCT) content into the blood. The transgenic pigs expressing rhEPO in their blood gave rise to higher RBC numbers and HCT contents than control animals. rhEPO was secreted both in the blood and milk of genetically engineered pigs harboring rhEPO gene. Therefore, this study provides a model regarding the production of transgenic pig carrying hEPO transgene for biomedical research.

This study was carried out to find out the changes on serum concentrations of estradiol-17β, progesterone in primiparous Duroc, Landrace and Yorkshire sows weaned at 7 or 21 days. Also, we compared the litter size at birth and weaning among the breeds weaned after lactation for 7 or 21 days. The estradiol-17β concentrations among the breeds were 6.9∼8.8 pg/ml and 6.4∼8.8 pg/ml after lactation for 7 or 21 days, respectively. The progesterone concentrations ranged from 0.3 ng/ml to 1.6 ng/ml. Duroc sow showed higher progesterone concentration compared with Landrace and Yorkshire sows weaned after lactation for 7 or 21 days. Also, we found out that litter size at birth and weaning, respectively, did not show any differences between day 7 and day 21 of lactation. From the facts mentioned above, it was suggested that very early weaning systems could work with no apparent adverse effect on prolificacy.

본 연구는 xanthine(X)-xanthine oxidase(XO) system하에서 돼지 난자의 체외성숙과 체외수정에 대한 catalase의 영향을 검토하였다. 그 결과 돼지 난포난자가 X 또는 XO하에서 배양되었을 때, 난포난자의 성숙율은 다른 배양시간에도 불구하고 catalase 첨가 유무에 따른 유의적인 차이를 나타내지 않았다. 그렇지만, X-XO-catalase system하에서 배양한 경우 유의적으로 높은 성숙율을 얻었다(P<0.05). 퇴행난자의 비율은 배양기간이 늘어남에 따라 증가되었으며, 배양 120시간에서는 catalase 첨가시보다 무첨가시에 유의적으로 높았다. 다른 한편으로, 단위발생 난자들이 배양 72시간에 높은 비율로 관찰되었지만, 다양한 배양시간에서 catalase 첨가유무에 따른 차이는 발견되지 않았다. 또 다른 실험에서, 동결-응해된 돼지 정자가 체외수정을 위해 X-XO system으로 처리되었다. 난자투명대에 대한 정자침입율은 none (P<0.05), XO, X+XO하에서 체외수정시 catalase 무첨가시보다 첨가시에 높게 나타났다. 다른 한편으로, 돼지정자가 none, X, XO, X+XO로 처리되었을 때, lipid peroxidation은 catalase 첨가시보다 무첨가시에 높은 비율로 나타났으며, 그 결과 정자침입과 lipid peroxidation에서의 변화가 상반되는 양상을 보였다. 그렇지만, 모든 조건하에서 정자의 sulfhydry (-SH) group의 함량은 catalase 첨가시에 높게 측정되었다. 난자의 투명대에 대한 정자의 접착 정도는 salt-stored 돼지 난자에 대한 정자접착을 통해서 평가되었으며, control group의 경우 X, XO, X+XO group에 비해 높은 정자접착율이 관찰되었다. 그렇지만, catalase 첨가유무에 따른 유의적인 차이는 인정되지 않았다. 본 연구의 결과는 X-XO-catalase system에 대한 난포난자와 정자의 노출이 돼지에서의 체외성숙과 체외수정을 촉진시키는 것으로 생각된다.

인체 트롬보포이에틴(hTPO)은 megakaryopoiesis 과정에 주요한 역할을 하는 사이토카인이다. 따라서 이러한 트롬보포이에틴을 유선조직에서 직접적으로 발현시키기 위하여 소 베타 카제인 프로모터, 인체 트롬보포이에틴 cDNA 및 네오유전자로 구성된 발현벡터를 구축하였다. 소 귀조직 세포로부터 유도된 섬유아세포에 lipoffctamine을 이용하여 발현벡터(pBT-L n대)의 삽입을 유도하였다. G4l8 저항성을 지닌 세포의 콜로니 형성을 유도하기 위하여 2주 이상 배양을 실시하였다. 형질전환 콜로니는 PCR에 의해 동정하였으며, 이들 콜로니를 핵치환 전까지 계속적으로 증식을 유도하였다. 형질전환 세포에 의해 재구성된 난자는 전기적인 융합과 calcium ionophore와 6-DMAP를 이용한 활성화를 실시하였으며, 체외에서 7일간 배양을 실시하였다. 총 35개의 콜로니를 PCR에 의해 분석한 결과, 이 중 29(82.9%)개가 형질전환된 콜로니였다. 형질전환된 세포로 재구성된 난자의 난할율 및 배반포로의 발달율은 65.1%와 23.8%로 나타났다. 형질전환된 세포로 재구성된 난자로부터 발달한 29개의 배반포 중 27개가 형질전환으로 확인되었다. 따라서 이러한 결과들은 형질전환 소 수정란을 형질전환된 세포를 이용한 체세포 복제 기법을 통해 효과적으로 생산할 수 있다는 것을 제시하고있다.