• 생명과학회지
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• 제34권1호
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• pp.48-58
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• 2024

살모넬라는 일반적으로 식품에 의해 전파되고 심각한 공중보건 문제를 야기하는 병원성 미생물로, 살모넬라에 대한 숙주의 감수성을 결정하는데 숙주의 유전적 요소가 중요한 역할을 담당한다. Cysteine-rich intestinal protein1 (CRIP1)은 LIM/double zinc finger protein family에 속하는 단백질로, 인간의 소화관과 폐, 비장을 포함한 인체 전반적인 부위에서 폭넓게 발현된다. 최근 CRIP1은 여러 면역 질환의 핵심적인 마커로서 보고되고 있지만, 숙주의 세균 감염에 대한 CRIP1의 영향은 아직 알려진 바가 없다. 살모넬라는 CRIP1 유전자를 굉장히 높은 수준으로 발현하는 소장의 파이엘반 내로 침입한다고 잘 알려져 있기 때문에, 본 연구에서는 살모넬라 감염과 CRIP1 결핍 간의 상관관계를 규명하는 것을 목표로 하였다. 우리는 ex vivo 분화 실험을 통해서 CRIP1 결핍은 골수-유래 대식세포의 식세포작용과 골수-유래 수지상세포의 보조자극 인자의 활성을 변화시키지 않는다는 것을 발견하였다. 게다가, 유세포 분석 데이터를 통해 야생형 마우스와 CRIP1 유전자 결핍 마우스 간의 MHCII⁺CD11b⁺ CD11c⁺ 수지상세포 및 MHCII⁺F4/80⁺CD11b⁺ 대식세포가 비슷한 수준을 나타낸다는 것을 보여주었다. 흥미롭게도, 비장의 단핵구와 장간막 림프절의 호중구의 기저 수준은 야생형 마우스보다 CRIP1 유전자 결핍 마우스에서 더욱 풍부하게 나타났다. 요약하자면, 우리는 CRIP1이 Salmonella Typhimurium 감염에 대한 숙주의 감수성과 골수성 세포의 활성에 불필요한 유전자임을 명확하게 증명하였다. 또한, 항원에 노출되지 않은 CRIP1 유전자 결핍 마우스에서 나타난 면역세포의 각기 다른 비율은 CRIP1 유전자의 발현 조절이 다양한 감염성 질환에 대한 새로운 면역치료 접근법일 수 있음을 시사한다.

• BMB Reports
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• 제44권2호
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• pp.123-128
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• 2011

Leucine-rich repeat containing protein 10 (LRRC10) is characterized as a cardiac-specific gene, suggesting a role in heart development and disease. A severe cardiac morphogenic defect in zebrafish morphants was recently reported but a contradictory result was found in mice, suggesting a more complicated molecular mechanism exists during mouse embryonic development. To elucidate how LRRC10 is regulated, we analyzed the 5'enhancer region approximately 3 kilo bases (kb) upstream of the Lrrc10 start site using luciferase reporter gene assays. Our characterization of the Lrrc10 promoter indicates it possesses complicated cis-and trans-acting elements. We show that GATA4 and MEF2C could both increase transcriptional activity of Lrrc10 promoter individually but that they do not act synergistically, suggesting that there exists a more complex regulation pattern. Surprisingly, knockout of Gata4 and Mef2c binding sites in the 5’enhancer region (-2,894/-2,889) didn't change the transcriptional activity of the Lrrc10 promoter and the likely GATA4 binding site identified was located in a region only 100 base pair (bp) upstream of the promoter. Our data provides insight into the molecular regulation of Lrrc10 expression, which probably also contributes to its tissue-specific expression.

• Clinical and Experimental Reproductive Medicine
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• 제26권1호
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• pp.103-109
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• 1999

Objective: Heat shock protein 70-2 (Hsp70-2) gene knockout mice are found to have premeiotic arrest at the primary spermatocyte stage with a complete absence of spermatids and spermatozoa. This observation led to the hypothesis that hspA2 may be disrupted in human testes with abnormal spermatogenesis. To test this hypothesis, we studied the mRNA expression of hspA2 in infertile men with azoospermia. Design: The mRNA expression were analyzed by competitive RT-PCR among testes with normal spermatogenesis, pachytene spermatocyte arrest, and sertoli-cell only syndrome. Materials and methods: Testicular biopsy was performed in men with azoospermia (n=15). Specimens were subdivided into three groups: (group 1) normal spermatogenesis (n=5), (group 2) spermatocyte arrest (n=5), (group 3) Sertoli-cell only syndrome (n=5). Total RNA was extracted by Trizol reagent. Total extracted RNA was reverse transcribed into cDNA and amplified by PCR using specific primers for hspA2 target cDNAs. A competitive cDNA fragment was constructed by deleting a defined fragment from the target cDNA sequence, and then coamplified with the target cDNA for competitive PCR. Glyceraldehyde-3-phosphate dehydrogenase (GAPDH) gene was used as an internal control. Results: On Competitive RT-PCR analyses for hspA2 mRNA, significant amount of hspA2 expression was observed in group 1, whereas a constitutively low level of hspA2 was expressed in groups 2 and 3. Conclusion(s): The study demonstrates that the hspA2 gene expression is down-regulated in human testes with abnormal spermatogenesis, which in turn suggests that hspA2 gene may play a specific role during meiosis in human testes.

• Molecules and Cells
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• 제41권8호
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• pp.742-752
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• 2018

Parkinson's disease (PD) is a neurodegenerative disease characterized by progressive degeneration of dopaminergic (DAergic) neurons, particularly in the substantia nigra (SN). Although circadian dysfunction has been suggested as one of the pathophysiological risk factors for PD, the exact molecular link between the circadian clock and PD remains largely unclear. We have recently demonstrated that $REV-ERB{\alpha}$, a circadian nuclear receptor, serves as a key molecular link between the circadian and DAergic systems. It competitively cooperates with NURR1, another nuclear receptor required for the optimal development and function of DA neurons, to control DAergic gene transcription. Considering our previous findings, we hypothesize that $REV-ERB{\alpha}$ may have a role in the onset and/or progression of PD. In the present study, we therefore aimed to elucidate whether genetic abrogation of $REV-ERB{\alpha}$ affects PD-related phenotypes in a mouse model of PD produced by a unilateral injection of 6-hydroxydopamine (6-OHDA) into the dorsal striatum. $REV-ERB{\alpha}$ deficiency significantly exacerbated 6-OHDA-induced motor deficits as well as DAergic neuronal loss in the vertebral midbrain including the SN and the ventral tegmental area. The exacerbated DAergic degeneration likely involves neuroinflammation-mediated neurotoxicity. The $REV-erb{\alpha}$ knockout mice showed prolonged microglial activation in the SN along with the over-production of interleukin $1{\beta}$, a pro-inflammatory cytokine, in response to 6-OHDA. In conclusion, the present study demonstrates for the first time that genetic abrogation of $REV-ERB{\alpha}$ can increase vulnerability of DAergic neurons to neurotoxic insults, such as 6-OHDA, thereby implying that its normal function may be beneficial for maintaining DAergic neuron populations during PD progression.

• 한국발생생물학회지:발생과생식
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• 제12권1호
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• pp.77-86
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• 2008

본 연구에서는 LIF의 첨가가 분리된 할구 유래의 생쥐 배아줄기세포 확립에 미치는 영향을 살펴보았다. 과배란 유도된 BDF1 생쥐로부터 2-세포기의 배아를 회수하여 각기 LIF가 첨가되지 않은 배양액과 1,000, 2,500, 5,000 U/mL의 LIF가 첨가된 배양액에서 포배기 배아까지 배양하였다. 배양된 포배기 배아는 차별화 염색 방법을 이용하여 내세포괴와 영양외배엽의 수를 계수하였다. 2,500 U/mL의 LIF 첨가 시 대조군($21.0{\pm}4.0$ vs. $15.9{\pm}5.0$, P<0.01)과 1,000 U/mL의 LIF를 처리한 군($21.0{\pm}4.0$ vs. $16.6{\pm}4.9$, P<0.05)에 비해서 내세포괴의 수가 유의하게(P<0.05) 증가하였다. 배아줄기세포주 확립 배양액으로는 FBS 대신 20% KSR과 0.01 mg/mL의 ACTH를 사용하였다. 2,500 U/mL의 LIF를 첨가 시 배아줄기세포 확립 효율이 36.7%(11/30)로 가장 높은 효율을 나타내었다. 이러한 배양 조건을 기본으로 하여 2-와 4-세포기 배아의 단일 할구를 분리하여 각기 21.4%(3/14)와 4.0%(1/20)의 효율로 단일 할구 배아줄기세포주를 확립할 수 있었다. 단일 할구로부터 확립된 배아줄기세포주와 이들에서 분화된 배아체는 세포면역학적 염색 방법과 RT-PCR 방법을 통해 그들의 미분화 특성과 삼배엽성 분화 특성을 확인할 수 있었다. 결론적으로 배양액에 LIF를 첨가하여 포배기 배아의 내세포괴 수를 증가시킬 수 있었으며, 분리된 할구의 배아줄기세포주 확립 효율을 향상시킬 수 있었다.