As an employee at  equipment manufacturer company (we also have developed some fluorescence readers) I can tell this is probably due to in the machine's inability to measure very bright signal. The fluorescence is being read by a sensor/camera with certain light exposure time, usually set in miliseconds. Those cameras/sensor usually have 3 dynamic ranges or Log10(3). This means by default you can read 10,100,1000 relative fluorescence units, this also means that you can trust the results only from 1-1000 RFU, results bigger than 1000 RFU are out of the dynamic range and 2000 RFU 3000 RFU or even 10000000 RFU are "equally" bright for the sensor or if to say simply, fluorescent light is blinding the sensor, so if you see a plateaued this can mean that the machine cannot see more. But manufacturers, in the pursuit of improving specifications of their machines, are playing with the exposure time, so if the sample is too bright they just switch to a lower exposure time, as maybe in your case the sample was so bright that the machine put it on the lower log and did not notice it.

Why it does not happen during qPCR? Cycling is the limiting factor: with each cycle total amount of DNA doubles. But NASBA is an avalanche type reaction and you would receive much more Nucleic Acid in comparison to qPCR, so in a result much brighter fluorescence signal.

But don't worry, the machine is working fine, maybe add less fluorescence marker in your sample.

That's a very interesting answer and something that I would not have thought of. Thank you very much.