伏隔核 D1 型中间神经元在标志追踪的表达和消退中的作用。
Role of nucleus accumbens D1-type medium spiny neurons in the expression and extinction of sign-tracking.
机构信息
Neuroscience Graduate Program, University of Michigan, Ann Arbor, MI 48109, USA; Department of Behavioral Neuroscience, Oregon Health and Science University, Portland, OR 97239, USA.
Rat Resource and Research Center, Animal Modeling Core, Veterinary Pathobiology, University of Missouri, Columbia, MO 65201, USA.
出版信息
Behav Brain Res. 2024 Feb 29;459:114768. doi: 10.1016/j.bbr.2023.114768. Epub 2023 Nov 18.
While sign-tracking, also known as autoshaping, has been studied for many decades, only recently has the tendency to show sign-tracking behavior been linked to the development and persistence of addiction. Sign-tracking is dependent upon dopamine activity in the nucleus accumbens (NAc). The NAc is comprised predominantly of medium spiny projection neurons (MSN) that can be differentiated by their D1-like or D2-like dopamine receptor expression. Here we determined how reducing activity of D1-type MSNs in the NAc affects the expression and extinction of sign-tracking. To address this, we transfected the NAc of transgenic male and female rats that selectively express Cre recombinase in D1-type MSNs with a DIO viral vector expressing hM4Di. Cre- rats were given the same viral infusion but did not express the hM4Di receptor and therefore served as controls. Rats were then conditioned to associate lever presentations with pellet delivery. After sign-tracking was established, all rats were administered clozapine-n-oxide (CNO) prior to three additional conditioning sessions to assess the effects of NAc D1-MSNs inhibition on sign-tracking in the presence of reward. CNO treatment did not alter the expression of sign-tracking in Cre+ or Cre- rats. Next rats underwent extinction training where lever presentations occurred without pellet delivery and all rats received a CNO injection prior to each extinction session. In these extinction conditions, Cre+ rats exhibited robust extinction of sign-tracking across sessions, whereas Cre- rats did not. To determine if D1-MSN inhibition merely produced a temporary cessation of sign-tracking or instead had facilitated a persistent loss of sign-tracking, we evaluated the reemergence of sign-tracking in a test for reconditioning. During testing, reintroduction of the CS-US pairing did not promote the reemergence of sign-tracking in Cre+ rats, but restored sign-tracking in Cre- rats. Thus, chemogenetic inhibition of NAc D1-MSNs promoted extinction of sign-tracking. Collectively, these data suggest that D1-MSNs play an important role in resistance to extinction that typifies sign-tracking behavior.
尽管标志跟踪(也称为自动塑造)已经研究了几十年,但直到最近,表现出标志跟踪行为的趋势才与成瘾的发展和持续有关。标志跟踪依赖于伏隔核(NAc)中的多巴胺活动。NAc 主要由中脑投射神经元(MSN)组成,这些神经元可以通过其 D1 样或 D2 样多巴胺受体表达来区分。在这里,我们确定了减少 NAc 中 D1 型 MSN 的活性如何影响标志跟踪的表达和消退。为了解决这个问题,我们用表达 hM4Di 的 DIO 病毒载体转染了选择性在 D1 型 MSN 中表达 Cre 重组酶的转基因雄性和雌性大鼠的 NAc。Cre-大鼠接受了相同的病毒输注,但不表达 hM4Di 受体,因此作为对照。然后,大鼠被训练将杠杆呈现与药丸传递联系起来。在建立标志跟踪后,所有大鼠在进行三次额外的条件训练之前,都给予氯氮平-N-氧化物(CNO),以评估 NAc D1-MSN 抑制对存在奖励时标志跟踪的影响。CNO 处理并未改变 Cre+或 Cre-大鼠标志跟踪的表达。接下来,大鼠进行消退训练,在没有药丸传递的情况下出现杠杆呈现,并且所有大鼠在每次消退训练之前都接受 CNO 注射。在这些消退条件下,Cre+大鼠在整个消退过程中表现出明显的标志跟踪消退,而 Cre-大鼠则没有。为了确定 D1-MSN 抑制是否只是暂时停止了标志跟踪,或者是否促进了标志跟踪的持久丧失,我们在重新条件训练的测试中评估了标志跟踪的重新出现。在测试期间,重新引入 CS-US 配对并没有促进 Cre+大鼠标志跟踪的重新出现,但恢复了 Cre-大鼠的标志跟踪。因此,NAc D1-MSN 的化学遗传抑制促进了标志跟踪的消退。总的来说,这些数据表明 D1-MSN 在抵抗标志跟踪行为所特有的消退方面发挥着重要作用。
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