• Asian-Australasian Journal of Animal Sciences
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• 제24권6호
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• pp.881-887
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• 2011

Feathers are one of the integument appendages that form the outer covering, or plumage, on birds. The goslings hatch with a downy coat of feathers formed in embryonic development. They moult the natal plumage into juvenile feathers between 3-5 weeks of age and than moult that juvenile plumage into adult plumage between 8-11 weeks of age. Feather weight of an adult goose makes up about 6.2% of its total body weight. Heritability of the feather production ability is relatively low ($h^2$ = 0.35). Within species or genotype, the quantity and composition of the plumage are affected by genetics (age, body weight or body surface area, feathering rate, sex) and environmental factors (nutrition and production system, weather, microclimate). After slaughter some 90-220 g marketable feathers can be obtained per goose. The yield of feathers and down from each hand-harvesting amounts to between 80 to 120 g per goose, depending upon the frequency and degree of completeness of the harvesting.

• 한국수정란이식학회지
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• 제14권1호
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• pp.6-15
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• 1999

ES cell의 수립으로 특히 mouse를 중심으로 한 발생학, 유전학 연구의 획기적 발전과 형질변환 동물의 생산 및 동물 체내에서 유전자 기능의 탐구에 매우 큰 변혁을 가져오게 되었다. 또한 ES cell과 embryoid body는 체외 분화능의 연구에 있어 새로운 cytokine의 발견 및 세포 수준에서의 유전자 기능 해석의 강력한 연구수단으로서 폭 넓게 이용되어 질 수 있는 가능성을 시사하고 있다. 이는 ES cell line이 지닌 두 가지 장점, 즉, 유전자 조작의 용이함과, 거의 모든 종류의 성체 구성세포로 분화할 수 있는 성질 때문이다. 이러한 ES cell technology를 실제로 제반 학문과 특히, 인간에게 적용하기 위해서는 반드시 해결해야 할 중요한 문제점이 있다. 첫째로, ES cell을 대상으로 하는 형질변환 방법의 편의성 및 효율개선이 이루어 wu야 하며, 두 번째로 인간의 유전자 및 세포 이식 치료 등을 비롯한 제반 연구에 직접 적용 가능한 ES cell line의 수립과 체외에서 목적으로 하는 분화 세포를 얻기 위한 배양조건이 확립되어져야 한다. 이러한 목표를 달성하기 위해 ES cell의 발생, 분화과정에 있어서의 분자조절기구, 세포 특이적 promotor, 유도 signal등에 대한 연구가 활발히 진행되어져야 할 것이다.

• Asian-Australasian Journal of Animal Sciences
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• 제6권3호
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• pp.447-450
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• 1993

The effect of adding transparent fluid (TF) to fowl semen on fertilizing capacity of fowl spermatozoa and on hatchability was studied. Diluted semen and semen containing 15% TF were stored for 24 h at $3-5^{\circ}C$ and inseminated at weekly basis for 5 consecutive weeks. No significant differences were observed in fertility, hatchability and embryonic mortality among the treatments. The results suggest that TF is not necessarily detrimental to fowl spermatozoa even when mixed with semen and stored outside the body.

• 대한지역사회영양학회:학술대회논문집
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• 대한지역사회영양학회 2005년도 춘계학술대회
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• pp.145-146
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• 2005

• Animal Bioscience
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• 제35권8호
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• pp.1223-1234
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• 2022

Objective: The objectives of this study were to evaluate the effects of daily feed intake during the laying period on embryonic myogenic differentiation 1 (MYOD1), myogenic factor 5 (MYF5), and myogenic factor 6 (MYF6) gene expression in genetically fat and lean lines of chickens. Methods: An experiment in a 2×2 factorial design was conducted with two dietary intake levels (100% and 75% of nutrition recommendation) and two broiler chicken lines (fat and lean). Two lines of hens (n = 384 for each line) at 23th week of age were randomly divided into 4 treatments with 12 replicates of 16 birds. The experiment started at 27th week of age (5% egg rate) and ended at 54th week of age. Hatched eggs from the medium laying period were collected. Real time polymerase chain reaction analysis was used to analyse the MYOD1, MYF5, and MYF6 mRNA levels of E7, E9, E11, E13, and E15 body tissues and E17, E19, and E21 chest and thigh muscle samples. Results: The results indicated that there were significant effects of line, dietary intake, and interactions between them on MYOD1, MYF5, and MYF6 gene mRNA expression levels in embryonic tissues. Low daily feed intake did not change the expression trend of MYOD1 mRNA in either line, but changed the peak values, especially in lean line. Low daily feed intake altered the trend in MYF5 mRNA expression level in both lines and apparently delayed its onset. There was no apparent effect of low daily feed intake on the trends of MYF6 mRNA expression levels in either line, but it significantly changed the values on many embryonic days. Conclusion: Maternal nutrient restriction affects myogenesis and is manifested in the expression of embryonic MYOD1, MYF5, and MYF6 genes. Long term selection for fat deposition in broiler chickens changes the pattern and intensity of myogenesis.

• Reproductive and Developmental Biology
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• 제32권4호
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• pp.223-227
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• 2008

Human embryonic stem (ES) cells retain the capacity for self-renewal, are pluripotent and differentiate into the three embryonic germ layer cells. The regulatory transcription factors Oct4, Nanog and Sox2 play an important role in maintaining the pluripotency of human ES cells. The aim of this research was to identify unknown genes upregulated in human ES cells along with Oct4, Nanog, and Sox2. This study characterizes an unknown gene, named chromosome 1 open reading frame 31 (C1orf31) mapping to chromosome 1q42.2. The product of C1orf31 is the hypothetical protein LOC388753 having a cytochrome c oxidase subunit VIb (COX6b) motif. In order to compare expression levels of C1orf31 in human ES cells, human embryoid body cells, vascular angiogenic progenitor cells (VAPCs), cord-blood endothelial progenitor cells (CB-EPCs) and somatic cell lines, we performed RT-PCR analysis. Interestingly, C1orf31 was highly expressed in human ES cells, cancer cell lines and SV40-immortalized cells. It has a similar expression pattern to the Oct4 gene in human ES cells and cancer cells. Also, the expression level of C1orf31 was shown to be upregulated in the S phase and early G2 phase of synchronized HeLa cells, leading us to purpose that it may be involved in the S/G2 transition process. For these reasons, we assume that C1orf31 may play a role in on differentiation of human ES cells and carcinogenesis.

• Molecules and Cells
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• 제23권1호
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• pp.49-56
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• 2007

One of the goals of stem cell technology is to control the differentiation of human embryonic stem cells (hESCs), thereby generating large numbers of specific cell types for many applications including cell replacement therapy. Although individual hESC lines resemble each other in expressing pluripotency markers and telomerase activity, it is not clear whether they are equivalent in their developmental potential in vitro. We compared the developmental competence of three hESC lines (HSF6, Miz-hES4, and Miz-hES6). All three generated the three embryonic germ layers, extraembryonic tissues, and primordial germ cells during embryoid body (EB) formation. However, HSF6 and Miz-hES6 readily formed neuroectoderm, whereas Miz-hES4 differentiated preferentially into mesoderm and endoderm. Upon terminal differentiation, HSF6 and Miz-hES6 produced mainly neuronal cells whereas Miz-hES4 mainly formed mesendodermal derivatives, including endothelial cells, leukocyte progenitors, hepatocytes, and pancreatic cells. Our observations suggest that independently-derived hESCs may differ in their developmental potential.

• 한국수정란이식학회지
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• 제6권1호
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• pp.33-40
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• 1991

In vitro developmental ability of early preimplantation monse embryos was shown to be depend on the embryonic stages, media and snpplements and their interaction(Experiment 1). The development of I-cell embryos were more promoted in the complex medinm(Ham's Fl0) than in the simple one(m-KRB), but that of 2-cell embryos showed the reverse effect. The bovine serum albumin(BSA) as a medium snpplement more promoted the development of I- and 2-cell embryos, compared with human fetal cord serum(HCS). On the other hand, the harmful effect of HCS was especially shown on the early cleavage in the embryonic development of the two stages. The effect of serum, in the respect of interaction between media and snpplements. was also more significantly appeared in m-KRB than Ham's Fl0. In the experiment 2, when the harmful effect of HCS was compared with that of fetal bovine serum(FBS), the former more promoted the development of l - and 2-cell embryos than the latter. The effect of HCS was more significantly shown in the development of I-cell than that of 2-cell embryos. Conclusively, as I- and 2-cell embryos were different in the requirements for the in vitro development. the optimal medium and supplement have to be selected for each embryonic stage. It is also respected to the better result if it take into consideration into the kinds of sera when serum is used for culture of early preimplantation embryos.

• 한국동물학회지
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• 제39권3호
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• pp.239-247
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• 1996

현탁 배양액에서 생쥐 배아주 세포를 배아체(embryoid body. EB)로 분화시키는 간단한 시험내 모델 체계가 초기 적혈구 분화 분석에 유용한 지의 여부를 조사하였다. 분화중인 배아체로부터 각 혈구계열 세포 유형이 만들어지는 지(분화능)의 여부는 혈도형성, benzidine 염색법 및 2단계 콜로니 분석법을 조사하였고, 발생과 분화시기에 바ㅈ추어 적혈구 표시 유전자들이 발현되는 지(발현능)의 여부는 각 분화시기별 배아체로 부터 추출한 RNA를 RT-PCR 방법으로 조사하였다. 분석 결과, 다른 기존의 복잡한 분화 방법에 의한 것과 마찬가지로 모든 혈구계열 세포 유형이 반복성 있게 유도되었다. 더군다나, 분화중인 배아주 세포에서의 글로빈 유전자 발현 전환은 생쥐 배아에서와 유사하게 진행되었으며, 글로빈 유전자의 발현은 적혈구-특이 전사인자인 GATA-1과 Tal-1보다 적어도 12시간 늦게 활성화되었다. 이와같이 간단한 분화 체계에서도 적혈구 분화과정이 효율적으로 반복성 있게 나타나는 것으로 보아, 간단한 현탁배양에서의 분화는 초기 적혈구 분화과정이 분자적 기작을 분석하는데 유용하게 이용될 수 있으리라 본다.

• 한국가축번식학회지
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• 제26권4호
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• pp.377-384
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• 2002

To investigate the expression patterns of proteins and growth factor signals in differentiated rabbit embryonic stem (ES) cells, ES cells with confluent stage grown of feeder layer and differentiated cells into embryoid bodies (EB) without feeder cell were applied to protein gel and Western blotting analysis. There were 66kDa and 28kDa specifically expressed in differentiated ES cell but not in undifferentiated ES cell while 25kDa protein band showed up in only undifferentiated ES cells. Also there were some difference of protein bands in several area of gel between differentiated and undifferentiated ES cells such as about 100 kDa, 50kDa and 27kDa areas, but there was no difference in band pattern of one-dimensional gel analysis between mouse ES cells and rabbit ES cells. IGF-I receptor and EGF receptor were expressed in differentiated cells and undifferentiated cells. And ICF-I and EGF were not expressed in both differentiated and undifferentiated cells. These results indicated that ES cells express their own proteins to inhibit differentiation while EB cells synthesize different proteins to differentiate, and 16F-I receptor and EGF receptor were expressed in both ES and EB cells probably for the different functions.